Abstract:
Disclosed are novel bactericidal/permeability-increasing (BPI) protein products wherein cysteine residue number 132 or 135 is replaced by another amino acid residue, preferably an alanine or serine residue and/or wherein the leucine residue at position 193 is the carboxy terminal residue. Also disclosed are DNA sequences encoding methods for the production of the same in appropriate host cells, and stable homogeneous pharmaceutical compositions containing the analogs suitable for use treatment of gram negative bacterial infection and its sequelae.

Description:
BACKGROUND OF THE INVENTION  
         [0001]    The present invention provides novel bactericidal/permeability-increasing protein products and stable pharmaceutical compositions containing the same.  
           [0002]    Lipopolysaccharide (LPS), is a major component of the outer membrane of gram-negative bacteria and consists of serotype-specific O-side-chain polysaccharides linked to a conserved region of core oligosaccharide and lipid A. Raetz,  Ann. Rev. Biochem.,  59:129-170 (1990). LPS is an important mediator in the pathogenesis of gram-negative septic shock, one of the major causes of death in intensive-care units in the United States, Morrison, et al.,  Ann. Rev. Med.  38:417-432 (1987).  
           [0003]    LPS-binding proteins have been identified in various mammalian tissues. Morrison,  Microb. Pathol.  7:389-398 (1989); Roeder, et al.,  Infect. Immun.,  57:1054-1058 (1989). Among the most extensively studied of the LPS-binding proteins is bactericidal/permeability-increasing protein (BPI), a basic protein found in the azurophilic granules of polymorphonuclear leukocytes. Human BPI protein has been isolated from polymorphonuclear neutrophils by acid extraction combined with either ion exchange chromatography [Elsbach,  J. Biol. Chem.,  254:11000 (1979)] or  E. coli  affinity chromatography [Weiss, et al.,  Blood,  69:652 (1987)] and has potent bactericidal activity against a broad spectrum of gram-negative bacteria.  
           [0004]    While the BPI protein is cytotoxic against many gram-negative bacteria, it has no reported cytotoxic activity toward gram-positive bacteria, fungi, or mammalian cells. The amino acid sequence of the entire human BPI protein, as well as the DNA encoding the protein, have been elucidated in FIG. 1 of Gray, et al.  J. Biol. Chem.,  264:9505 (1989), incorporated herein by reference (SEQ ID NOs: 1 and 2). The Gray et al. publication discloses the isolation of human BPI-encoding cDNA from a cDNA library derived from DMSO-induced cells of the human promyelocytic leukemia HL-60 cell line (ATTC CCL 240). Multiple PCR amplifications of DNA from a freshly prepared cDNA library derived from such DMSO-induced HL-60 cells have revealed the existence of human BPI-encoding cDNAs wherein the codon specifying valine at amino acid position 151 is either GTC (as set out in SEQ ID No: 1) or GTG. Moreover, cDNA species employing GTG to specify valine at position 151 have also been found to specify either lysine (AAG) for the position 185 amino acid (as in SEQ ID Nos: 1 and 2) or a glutamic acid residue (GAG) at that position.  
           [0005]    A proteolytic fragment corresponding to the N-terminal portion of human BPI holoprotein possesses the antibacterial efficacy of the naturally-derived 55 kDa human BPI holoprotein. In contrast to the N-terminal portion, the C-terminal region of the isolated human BPI protein displays only slightly detectable anti-bacterial activity. Ooi, et al.,  J. Exp. Med.,  174:649 (1991). A BPI N-terminal fragment, comprising approximately the first 199 amino acids of the human BPI holoprotein, has been produced by recombinant means as a 23 kD protein. Gazzano-Santoro et al.,  Infect. Immun.  60:4754-4761 (1992).  
           [0006]    The projected clinical use of BPI products for treatment of gram-negative sepsis in humans has prompted significant efforts to produce large quantities of recombinant BPI (rBPI) products suitable for incorporation into stable, homogeneous pharmaceutical preparations. For example, co-owned, co-pending U.S. patent application Ser. No. 07/885,501 by Grinna discloses novel methods for the purification of recombinant BPI products expressed in and secreted from genetically transformed mammalian host cells in culture. Efficacy of the purification processes is therein demonstrated in the context of products of transformed CHO cells which express DNA encoding the 31 amino acid “leader” sequence of human BPI and the initial 199 amino terminal residues of the mature protein (i.e. corresponding to the amino acids −31 through 199 of SEQ ID NO: 2). Co-owned, co-pending U.S. patent application Ser. No. 07/885,911 by Theofan, et al. is directed to novel, recombinant-produced BPI protein analog products resulting from the expression of DNA encoding the BPI leader sequence and either 191 or 199 amino terminal residues of human BPI fused to DNA encoding a constant region of an immunoglobulin heavy chain.  
           [0007]    Efforts to produce pharmaceutical grade BPI products for treatment of gram negative sepsis in humans have not yielded uniformly satisfactory results. A principal reason for this is the nature of the amino acid sequence of human BPI and the nature of the recombinant host cell environment in which the products are produced. As one example, biologically-active rBPI products comprising the initial 199 residues of BPI [rBPI(1-199)] produced as secretory products of transfected CHO host cells may be purified in good yields. However, the isolated BPI products initially include dimeric forms of BPI as well as cysteine adduct species. Moreover, BPI products may be unstable upon storage at physiological temperature and pH, resulting in the formation of additional dimeric and adduct species. Such dimeric and adduct species, while retaining biological activity, are not preferred for incorporation into pharmaceutical preparations projected for human use. Dimer formation and the formation of cysteine adducts are the probable result of the fact that BPI includes three cysteine amino acid residues, all of which are positioned within the biologically active amino terminal region of BPI, i.e., at positions 132, 135 and 175. Formation of a single disulfide bond between two of the three cysteines allows for dimer formation or formation of cysteine adducts with the remaining free cysteine in the host cell cytoplasm and/or the cell culture supernatant.  
           [0008]    Even monomeric rBPI products display varying degrees of microheterogeneity in terms of the number of carboxy terminal residues present in such products. For example, it is difficult to detect full-length expression product in a medium containing host cells transformed or transfected with DNA encoding rBPI(1-199). Instead, the expression products obtained from such cells represent an heterogeneous array of carboxy-terminal truncated species of the rBPI N-terminal fragment. In fact, the expected full-length product (1-199) is often not detected as being among the rBPI species present in that heterogeneous array. Heterogeneity of the carboxy terminal amino acid sequence of rBPI(1-199) products appears to result from activity of carboxypeptidases in host cell cytoplasm and/or culture supernatant.  
           [0009]    An additional problem encountered in the preparation of pharmaceutical-grade BPI products is the formation of macroscopic particles which decrease the homogeneity of the product, as well as decreasing its activity. A preferred pharmaceutical composition containing rBPI products according to the invention comprises the combination of a poloxamer (polyoxypropylene-polyoxyethylene block copolymer) surfactant and a polysorbate (polyoxyethylene sorbitan fatty acid ester) surfactant. Such combinations are taught in co-owned, co-pending, concurrently-filed U.S. patent application Ser. No. (Attorney docket no. 27129/31162) to have synergistic effects in stabilizing pharmaceutically-active polypeptides against particle formation. Most preferred is a composition in which the rBPI product is present in a concentration of 1 mg/ml in citrate buffered saline (0.02 M citrate, 0.15 M NaCl, pH 5.0) comprising 0.1% by weight of poloxamer 188 (Pluronic F-68. BASF Wyandotte, Parsippany, N.J.) and 0.002% by weight of polysorbate 80 (Tween 80, ICI Amencas Inc., Wilmington, Del.).  
           [0010]    There continues to be a need in the art for improved rBPI products suitable for incorporation into stable homogeneous pharmaceutical preparations. Such products would ideally be obtainable in large yield from transformed host cells, would retain the bactericidal and LPS-binding biological activities of BPI, and would be limited in their capacity to form dimeric species and cysteine adducts, and would be characterized by limited variation in carboxy termini.  
         SUMMARY OF THE INVENTION  
         [0011]    The present invention provides novel, biologically-active, recombinant-produced BPI (“rBPI”) protein and protein fragment products which are characterized by a resistance to dimerization and cysteine adduct formation, making such products highly suitable for pharmaceutical use. Also provided are rBPI products characterized by decreased molecular heterogeneity at the carboxy terminus. Novel DNA sequences encoding rBPI products and analog products, plasmid vectors containing the DNA, host cells stably transformed or transfected with the plasmids, recombinant preparative methods, stable pharmaceutical compositions and treatment methods are also provided by the invention.  
           [0012]    According to one aspect of the present invention, rBPI protein analogs are provided which comprise a BPI N-terminal fragment wherein a cysteine at amino acid position 132 or 135 is replaced by another amino acid, preferably a non-polar amino acid such as serine or alanine. In a preferred embodiment of the invention, the cysteine residue at position 132 of a polypeptide comprising the first 199 N-terminal residues of BPI is replaced by an alanine residue in a recombinant product designated “rBPI(1-199)ala 132 ”. Also in a preferred embodiment of the invention, the cysteine at position 135 of a BPI fragment comprising the first 199 N-terminal BPI residues is replaced by a serine, resulting in a recombinant product designated “rBPI(1-199)ser 135 ”. Highly preferred is a recombinant product designated “rBPI(1-193)ala 132 ” which is characterized by decreased heterogeneity in terms of the identity of its carboxy terminal residue. Also in a preferred embodiment of the invention, a polypeptide is taught which comprises the first 193 amino-terminal residues of BPI and which has a stop codon immediately following the codon for leucine at position 193.  
           [0013]    According to another aspect of the invention, DNA sequences are provided which encode the above-described rBPI protein and protein fragment products, including analog products. Such DNA sequences may also encode the 31-residue BPI leader sequence and the BPI polyadenylation signal. Also provided are autonomously-replicating DNA plasmid vectors which include DNA encoding the above-mentioned products and analogs as well as host cells which are stably transformed or transfected with that DNA in a manner sufficient to allow their expression. Transformed or transfected host cells according to the invention are of manifest utility in methods for the large-scale production of rBPI protein products of the invention.  
           [0014]    The invention also contemplates rBPI protein analog products in the form of fusion proteins comprising, at the amino terminal, rBPI protein analog products of the invention and, at the carboxy terminal, a constant region of an immunoglobulin heavy chain or an allelic variant thereof. Natural sequence BPI/immunoglobulin fusion proteins are taught in the co-pending, co-owned U.S. patent application Ser. No. 07/885,911 by Theofan, et al., the disclosures of which are incorporated herein by reference. The invention further contemplates methods for producing the aforementioned fusion proteins.  
           [0015]    Also within the scope of the present invention are DNA sequences encoding biologically-active rBPI protein fragment products having from about 176 to about 198 of the N-terminal amino acids of BPI. These DNAs allow for production of BPI products in eucaryotic host cells, such as CHO cells, wherein the products display less heterogeneity in terms of the carboxy terminal residues present. Presently preferred are DNAs encoding 193 N-terminal residues of BPI (e.g., DNAs encoding the thirty-one amino acid leader sequence of BPI, the initial 193 N-terminal amino acids, and one of more step codons. Most preferred are such DNAs which additionally encode proteins wherein the cysteine at either position 132 or 135 is replaced (e.g. rBPI(1-193)ala 132 ).  
           [0016]    Finally, the present invention also provides stable, homogeneous pharmaceutical compositions comprising the rBPI protein products of the invention in pharmaceutically acceptable diluents, adjuvants, and carriers. Such pharmaceutical compositions are resistant to the formation of rBPI product particles. Such compositions are useful in the treatment of gram-negative bacterial infection and the sequelae thereof, including endotoxin-related shock and one or more conditions associated therewith, such as disseminated intravascular coagulation, anemia, thrombocytopenia, leukopenia, adult respiratory distress syndrome, renal failure, hypotension, fever, and metabolic acidosis.  
           [0017]    Numerous additional aspects and advantages of the invention will become apparent to those skilled in the art upon considering the following detailed description of the invention which describes presently preferred embodiments thereof. 
       
    
    
     BRIEF DESCRIPTION OF THE DRAWING  
       [0018]    [0018]FIG. 1 represents results of SDS-PAGE analysis of rBPI(1-199) products.  
         [0019]    [0019]FIG. 2 represents results of SDS-PAGE analysis of rBPI(1- 193) and rBPI(1-199)ala 132  products.  
         [0020]    [0020]FIG. 3 depicts results of cation exchange HPLC analysis of rBPI(1-199) products.  
         [0021]    [0021]FIG. 4 shows results of cation exchange HPLC analysis of rBPI(1-199)ala 132  products.  
         [0022]    [0022]FIG. 5 represents results of reverse phase HPLC run on rBPI(1-199) products.  
         [0023]    [0023]FIG. 6 represents results of reverse phase HPLC run on rBPI(1-199)ala 132  products.  
         [0024]    [0024]FIG. 7 presents results of turbidity studies on pharmaceutical compositions containing rBPI products with and without poloxamer/polysorbate surfactant ingredients at pH 7.0 and 57° C.  
         [0025]    [0025]FIG. 8 depicts comparative binding of rBPI(1-199) and rBPI(1-199)ala 132  to LPS.  
         [0026]    [0026]FIG. 9 reports the bactericidal activity of rBPI(1-199)ala 132  products. 
     
    
     DETAILED DESCRIPTION  
       [0027]    The following detailed description relates to the manufacture and properties of various rBPI product preparations which comprise an amino acid substitution at a cysteine residue and/or highly uniform carboxy termini. More specifically, Example 1 relates to an exemplary means by which base substitutions are introduced in the nucleotide sequence encoding an exemplary N-terminal fragment of the BPI protein and to the incorporation of such mutated sequences into plasmid vectors. Example 2 addresses the incorporation of vectors of Example 1 into appropriate host cells and further describes the expression of recombinant BPI protein polypeptide products of the invention. Example 3 relates to construction of DNAs encoding cysteine replacement analog products of the invention and the use thereof in in vitro transcription/translation procedures. Example 4 relates to properties of rBPI product polypeptides of the invention.  
       EXAMPLE 1  
     Construction Of Vectors Containing BPI Cysteine Replacement Analogs  
       [0028]    A. Construction of Plasmids pING4519 And pING4520  
         [0029]    The expression vector, pING4503, was used as a source of DNA encoding a recombinant expression product designated rBPI(1-199), i.e., encoding a polypeptide having the 31-residue signal sequence and the first 199 amino acids of the N-terminus of the mature human BPI, as set out in SEQ ID NOs: 1 and 2 except that valine at position 151 is specified by GTG rather than GTC and residue 185 is glutamic acid (specified by GAG) rather than lysine (specified by AAG).  
         [0030]    Plasmid pING4503 has been described in co-pending, co-owned U.S. patent application Ser. No. 07/885,911 by Theofan, et al. which is incorporated herein by reference with respect to the background of the invention. Briefly, the construction of pING4503 is based on plasmid pING2237N which contains the mouse immunoglobulin heavy chain enhancer element, the LTR enhancer-promoter element from Abelson murine leukemia virus (A-MuLv) DNA. the SV40 19S/16S splice junction at the 5′ end of the gene to be expressed, and the human genomic gamma-1 polyadenylation site at the 3′ end of the gene to be expressed. Plasmid pING2237N also has a mouse dihydrofolate reductase (DHFR) selectable marker. The DNA encoding rBPI(1-199), including 30 bp of the natural 5′ untranslated region and bases encoding the 31 amino acid signal sequence, as well as 199 N-terminal amino acids of BPI, is inserted between unique SAlI and SstII restriction sites in pING4503.  
         [0031]    Two vectors, pING4519 and pING4520, were constructed based on pING4503 for expression of rBPI(1-199) cysteine replacement analogs in which one of the three naturally-occurring cysteine residues of BPI was replaced with another amino acid. A PvuII site (CAGCTG) which occurs only once in the DNA encoding rBPI(1-199), and which is located between cysteine 132 and cysteine 135, was utilized in these constructions. Because several additional PvuII sites exist in pING4503, it was first necessary to isolate the SalI-SstII fragment which contained the insert encoding rBPI(1-199) from pING4503 by digesting with SalI and SstII. The purified SalI-SstII rBPI(1-199) insert was then digested with PvuII, resulting in an approximately 529 bp SalI-PvuII fragment and an approximately 209 bp PvuII-SstII fragment, each of which was purified separately.  
         [0032]    Plasmid pING4519 is identical to pING4503 except that pING4519 contains a DNA insert encoding an rBPI(1-199) in which a codon for alanine is substituted for the codon specifying the native cysteine at position 132. As noted above, the recombinant product resulting from host cell expression and secretory processing of such an insert is referred to as “rBPI(1-199)ala 132 ”. In order to generate pING4519, BPI DNA sequences were PCR amplified from pING4503 using the primers BPI-6: AAGCTTGTCGACCAGGCCTTGAGGT (SEQ ID NO: 3), which incorporated a SalI restriction site at the 5′ end of the 30 bp BPI untranslated region, and BPI-14: CTGGAGGCGGTGATGGTG (SEQ ID NO: 4), which incorporated one half of the PvuII site and the base substitutions necessary to code for alanine at position 132. PCR amplification was accomplished using the GeneAmp PCR kit (Perkin Elmer Cetus, Norwalk, Conn.) according to the manufacturer&#39;s instructions. The resulting PCR fragment was digested with SalI, resulting in an approximately 529 bp SalI-blunt fragment which was then used in a three-piece ligation, together with the approximately 209 bp PvuII-SstII fragment described above and the large fragment resulting from SalI and SstII digestion of pING4503, to generate pING4519.  
         [0033]    Plasmid pING4520 is identical to pING4519 with the exception that pING4520 contains a DNA insert encoding an rBPI(1-199) analog in which a serine codon is substituted for the codon specifying the native cysteine at position 135. As noted above, the recombinant product resulting from host cell expression of such an insert is designated “rBPI(1-199) ser 135 ”. In order to generate pING4520, BPI DNA sequences were PCR amplified from pING4513, a plasmid essentially similar to pING4503 except that the selection marker is gpt instead of DHFR and the cDNA insert encodes the signal sequence and full-length BPI (456 residues) instead of only the rBPI(1-199) portion.  
         [0034]    Amplification by PCR was accomplished using primer BPI-15: CTCCAGCAGCCACATCAAC (SEQ ID NO: 5), wherein the 5′ end incorporates one half of a mutated PvuII site (wherein “CTG” is changed to “CTC”) and the base substitutions necessary to code for serine at position 135; and primer BPI-7: GAACTTGGTTGTCAGTCG (SEQ ID NO: 6), representing rBPI-encoding sequences located downstream of the region encoding BPI residue 199. This PCR fragment was digested with BstBI, which cuts downstream of the cysteine 135 mutagenesis site, and the resulting approximately 100 bp blunt-BstBI fragment was gel purified. A three piece ligation was then performed with the 529 bp SalI-PvuII BPI restriction fragment described above, the 100 bp blunt-BstBI fragment, and a large fragment resulting from BstBI-SalI digestion of pING4503, to generate pING4520.  
         [0035]    B. Construction Of Plasmid pING4530  
         [0036]    Another vector, pING4530, was constructed which contained the alanine-for- cysteine replacement as in pING4519, but which contained the gpt selectable marker (allowing for mycophenolic acid resistance) instead of the DHFR marker carried over from pING4503 to pING4519. To construct pING4530, a 1629 bp SalI-DraIII restriction fragment was isolated from pING4519. This fragment included all of the rBPI(1-199)ala 132  coding region as well as an additional approximately 895 bp vector sequence at the 3′ end of the coding region. This fragment was ligated to the large (approximately 7230 bp) DraIII-SalI vector fragment isolated from pING4513 to generate pING4530.  
         [0037]    C. Construction Of Plasmid pING4533  
         [0038]    Plasmid pING4533 was constructed for expression of rBPI(1- 199)ala 132 , wherein the codon specifying the fifth amino acid of the BPI signal sequence. methionine (ATG), at position -27 was placed in the context of the consensus Kozak translation initiation sequence GCCACCRCCATGG (SEQ ID NO: 7) [Kozak,  Nucl. Acid. Res.,  15:8125 (1987)], and in which the DNA sequence encoding the first 4 amino acids of the BPI signal was removed. This was accomplished by PCR amplification of BPI sequences from a plasmid containing the full length human BPI cDNA [in pGEM-7zf(+)] using the PCR primer BPI-23: ACTGTCGACGCCACCATGGCCAGGGGC (SEQ ID NO: 8), incorporating a SalI restriction site and the nucleotides GCCACC in front of the ATG (methionine) at position −27 of the BPI signal, and the primer BPI-2: CCGCGGCTCGAGCTATATTTTGGTCAT (SEQ ID NO: 9), corresponding to the 3′ end of the rBPI(1-199) coding sequence.  
         [0039]    The approximately 700 bp PCR amplified DNA was digested with SalI and EcoRI and the resulting 270 bp fragment, including approximately the first one-third of the BPI(1-199) coding sequence, was purified. This SalI-EcoRI fragment was ligated to 2 other fragments: (1) a 420 bp EcoRI-SstII fragment from pING4519, encoding the remainder of BPI(1-199) wherein alanine replaces cysteine at position 132: and (2) an approximately 8000 bp SstII-SalI vector fragment from pING4502 (a vector essentially similar to pING4503 except that it does not include the 30 bp 5′ untranslated sequence and has a gpt marker rather than DHFR), to generate pING4533 which contains a gpt marker.  
         [0040]    D. Construction Of Plasmids pING4221, pING422, And pING4223  
         [0041]    Vectors similar to pING4533 were constructed having an insert which contained the optimized Kozak translation initiation site corresponding to methionyl residue −27 of the signal sequence, and an alanine-for-cysteine replacement at position 132. However, the BPI fragment coding sequence terminated at residue 193 in these constructions. As noted above, the recombinant product resulting from host cell expression of this DNA is referred to as “rBPI(1-193)ala 132 ”. Vectors containing these inserts were made by first digesting pING4533 with SalI, which cuts at the 5′ end of the BPI DNA insert, and AlwNI, which leaves a three bp 3′-overhang at residue 192. The resulting approximately 700 bp fragment was then purified. This fragment was re-ligated into the large fragment resulting from pING4523 digestion with SstII-SalI, along with two annealed complementary oligonucleotides, BPI-30: CTGTAGCTCGAGCCGC (SEQ ID NO: 10) and BPI-31: GGCTCGAGCTACAGAGT (SEQ ID NO: 11). This replaced the region between the AlwNI and SstII sites with the codon for residue 193 (leucine), a stop codon, and an XhoI restriction site 5′ to the SstIII site and resulted in regeneration of both the AlwNI and the SstII sites and placement of the stop codon, TAG, immediately after the codon (CTG) for amino acid 193 (leucine). The resultant plasmid was designated pING4223 and had the gpt marker. Similar constructions were made exactly as described for pING4223 except that different SstII-SalI vector fragments were used to generate vectors with different selection markers. For example, pING4221 is identical to pING4223 except that it contains the his marker (conferring resistance to histidinol) instead of gpt and pING4222 is identical to pING4223 except that it contains the DHFR marker instead of gpt.  
         [0042]    E. Construction Of Plasmids pING4537, pING4143. pING4146, pING4150, And pING4154  
         [0043]    A series of vectors was constructed which contained an insert encoding rBPI(1-193)ala 132 , the optimized Kozak translation initiation site, and different selection markers essentially identical to those described with respect to pING4221, pING4222 and pING4223 except that the human genomic gamma-1 heavy chain polyadenylation and transcription termination region at the 3′ end of the SstII site was replaced with a human light chain polyadenylation sequence followed by mouse light chain (kappa) genomic transcription termination sequences. In collateral gene expression studies, the light chain polyadenylation signal and transcription termination region appeared to be responsible for 2.5-5 fold increases in BPI expression levels in Sp2/0 and CHO-K1 cells.  
         [0044]    The aforementioned vectors were constructed by first constructing pING4537, a vector similar to pING4533 which contains the rBPI(1-199)ala 132  insert. However, pING4537 includes the human light chain polyadenylation sequences instead of the human heavy chain sequence. The mouse kappa 3′ sequences were obtained from pING3170, an expression vector which encodes a human light chain cDNA and includes a mouse genomic light chain 3′ transcription termination sequence. This was accomplished by digesting with SstI, which cuts 35 bp upstream of the mouse light chain stop codon, treating with T4 DNA polymerase to make the end blunt, then cutting with BamHI, and purifying an approximately 1350 bp fragment which includes the mouse kappa 3′ sequences. The resulting fragment consists of approximately 250 bp of the 3′ portion of the human light chain constant region cDNA and the polyadenylation signal followed by a BamHI linker as described in the construct called Δ8 in Lui et al.,  J. Immunol.  139: 3521, (1987). The remainder of the approximately 1350 bp fragment consists of a BglII-BamHI mouse kappa 3′ genomic fragment [fragment “D” of Xu et al.,  J. Biol. Chem.  261:3838, (1986)] which supplies transcription termination sequences. This fragment was used in a 3-piece ligation with two fragments from pING4533: a 3044 bp fragment which includes all of BPI insert and part of vector obtained by digestion with SstII, T4 polymerase treatment, and NotI digestion (which includes all of BPI insert and part of vector), and an approximately 4574 bp BamHI-NotI fragment. The resulting vector, pING4537, is identical to pING4533 with the exception of the above-noted differences in the genomic 3′ untranslated region.  
         [0045]    Additional vectors containing the kappa 3′ untranslated sequences were constructed using pING4537 as the source of the kappa 3′ fragment. The kappa 3′ untranslated sequences were isolated by digestion of pING4537 with XhoI (a unique site which occurs immediately after the BPI stop codon) and BamHI. The resulting approximately 1360 bp XhoI-BamHI fragment was used in a series of 3-piece ligations to generate the following four vectors, all of which have inserts encoding rBPI(1-193)ala 132  and which have the optimized Kozak translation initiation site at residue −27 of the signal: (1) pING4143 (gpt marker), obtained by ligating a pING4223 4574 bp BamHI-NotI fragment (gpt marker), a pING4223 NotI-XhoI BPI insert-containing fragment of approximately 3019 bp, and the pING4537 XhoI-BamHI fragment; (2) pING4146 (DHFR marker), obtained by ligating a pING4222 approximately 4159 bp BamHI-NotI fragment (DHFR marker), a pING4223 NotI-XhoI BPI insert-containing fragment of approximately 3019 bp, and the pING4537 XhoI-BamHI fragment; (3) pING4150 (his marker), obtained by ligating a pING4221 his-containing approximately 4772 bp BamHI-NotI fragment, a pING4222 NotI-XhoI BPI insert-containing fragment, and the pING4537 XhoI-BamHI fragment; and (4) pING4154 (neo marker), obtained by ligating a pING3174 neo-containing approximately 4042 bp BamHI-BsaI fragment, a pING4221 BsaI-XhoI BPI insert-containing fragment of approximately 3883 bp and the pING4537 XhoI-BamHI fragment. Plasmid pING3174 contains an insert encoding antibody heavy chain DNA and has a neo marker. The neo gene and its flanking sequences were obtained from the pSv2 neo plasmid reported by Southern et al.,  J. Mol. Appl. Genet.,  1:327 (1982).  
         [0046]    F. Construction Of Plasmids pING4144 And pING4151  
         [0047]    Two plasmids were constructed, pING4144 and pING4151, which were identical to pING4143 and pING4150, respectively, except that expression of rBPI coding sequences was under control of the human cytomegalovirus (hCMV) immediate early enhancer/promoter instead of the Abelson murine leukemia virus (A-MuLv) LTR promoter. Therefore, both pING4144 and pING4151 contained the mutation of the cysteine at position 132 to alanine, the optimized Kozak translation initiation sequence, and the human light chain poly-A/mouse kappa genomic transcription termination region. The region between nucleotides 879 and 1708 of the original vectors (pING4143 and pING4150) was replaced with a region of the hCMV enhancer/promoter corresponding to nucleotides −598 through +174 as shown in FIG. 3 of Boshart et al.,  Cell  41:521 (1985), incorporated herein by reference. To introduce the hCMV promoter region into BPI expression vectors, plasmid pING4538 was first constructed by replacing the approximately 1117 bp EcoRI-SalI/A-MuLv promoter-containing fragment of pING4212 with an approximately 1054 bp EcoRI-SalI/hCMV promoter-containing fragment from plasmid pING2250 which contains the hCMV promoter driving expression of an antibody light chain insert. To construct pING4144, three fragments were ligated together: (1) the approximately 2955 bp rBPI(1-193)-containing NotI-XhoI fragment from pING4538: (2) the approximately 1360 bp XhoI-BamHI fragment from pING4537; and (3) the approximately 4770 bp BamHI-NotI fragment containing the his gene from pING4221.  
         [0048]    G. Construction Of Plasmids pING4145, pING4148 And pING4152  
         [0049]    Plasmids pING4145, pING4148 and pING4152 were constructed and were identical to pING4143. pING4146, and pING4150, respectively, except that they contained the wild-type (natural sequence) cysteine at position 132 instead of an alanine substitution. Thus, all three contained the rBPI(1-193) insert, the optimized Kozak translation initiation sequence and the human light chain Poly A/mouse kappa genomic transcription termination region. These three plasmids were constructed as follows. To construct pING4145, three fragments were ligated together: (1) the approximately 3000 bp NotI-XhoI BPI(1-193) containing fragment from pING4140 (pING4140 is identical to pING4221 except that it contains the wild-type cysteine at Position 132); (2) the approximately 1360 bp XhoI-BamHI fragment from pING4537; and (3) the approximately 4570 bp BamHI-NotI fragment containing the gpt gene from pING4223. To construct pING4148, three fragments were ligated together: (1) the NotI-XhoI fragment from pING4140; (2) the XhoI-BamHI fragment from pING4537; and (3) the approximately 4150 bp BamHI-NotI fragment containing the DHFR gene from pING422. To construct pING4152, three fragments were ligated together: (1) the approximately 3000 bp NotI-XhoI fragment from pING4142 (pING4142 is identical to pING4223 except that it contains the wild-type cysteine at 132); (2) the XhoI-BamHI fragment from pING4537; and (3) the approximately 4770 bp BamHI-NotI fragment containing the his gene from pING4221.  
         [0050]    Table 1, below, summarizes the content of the plasmids whose preparation is described in Sections A through G above.  
                                                 TABLE I                                       Signal            Plasmid   BPI Product   Seq.   Marker   3′ Terminal   Promoter               pING4519   (1-199)Ala 132     31AA   DHFR*   Human   A-MuLv                       Genomic HC                       Gamma-1                       Poly-A       pING4520   (1-199)Ser 135     31AA   DHFR*   Human   A-MuLv                       Genomic HC                       Gamma-1                       Poly-A       pING4530   (1-199)Ala 132     31AA   gpt   Human   A-MuLv                       Genomic HC                       Gamma-1                       Poly-A       pING4533   (1-199)Ala 132     Kozak   gpt   Human   A-MuLv               initi-       Genomic HC               ation       Gamma-1               Seq;       Poly-A               27AA               signal       pING4223   (1-193)Ala 132     Kozak   gpt   Human   A-MuLv               initi-       Genomic HC               ation       Gamma-1               Seq;       Poly-A               27AA               signal       pING4221   (1-193)Ala 132     Kozak   his   Human   A-MuLv               initi-       Genomic HC               ation       Gamma-1               Seq;       Poly-A               27AA               signal       pING4222   (1-193)Ala 132     Kozak   DHFR   Human   A-MuLv               initi-       Genomic HC               ation       Gamma-1               Seq:       Poly-A               27AA               signal       pING4537   (1-199)Ala 132     Kozak   gpt   Human   A-MuLv               initi-       Kappa Poly-               ation       A/Mouse               Seq;       Kappa               27AA       Genomic               signal       Transcription                       Termination       pING4143   (1-193)Ala 132     Kozak   gpt   Human   A-MuLv               initi-       Kappa Poly-               ation       A/Mouse               Seq;       Kappa               27AA       Genomic               signal       Transcription                       Termination       pING4146   (1-193)Ala 132     Kozak   DHFR   Human   A-MuLv               initi-       Kappa Poly-               ation       A/Mouse               Seq;       Kappa               27AA       Genomic               signal       Transcription                       Termination       pING4150   (1-193)Ala 132     Kozak   his   Human   A-MuLv               initi-       Kappa Poly-               ation       A/Mouse               Seq;       Kappa               27AA       Genomic               signal       Transcription                       Termination       pING4144   (1-193)Ala 132     Kozak   gpt   Human   hCMV               initi-       Kappa Poly-               ation       A/Mouse               Seq;       Kappa               27AA       Genomic               signal       Transcription                       Termination       pING4145   (1-193)   Kozak   gpt   Human   A-MuLv               initi-       Kappa Poly-               ation       A/Mouse               seq;       Kappa               27AA       Genomic               signal       Transcription                       Termination       pING4148   (1-193)   Kozak   DHFR   Human   A-MuLv               initi-       Kappa Poly-               ation       A/Mouse               Seq;       Kappa               27AA       Genomic               signal       Transcription                       Termination       pING4152   (1-193)   Kozak   his   Human   A-MuLv               initi-       Kappa Poly-               ation       A/Mouse               Seq;       Kappa               27AA       Genomic               Signal       Transcription                       Termination       pING4151   (1-193)ala 132     Kozak   his   Human   hCMV               initi-       Kappa Poly-               ation       A/Mouse               Seq;       Kappa               27AA       Genomic               signal       Transcription                       Termination       pING4154   (1-193)ala 132     Kozak   neo   Human   A-MuLv               initi-       Kappa Poly-               ation       A/Mouse               Seq;       Kappa               27AA       Genomic               signal       Transcription                       Termination                          
 
       EXAMPLE 2  
     Transfection Of Cells For Expression of The rBPI Cysteine Replacement Analogs  
       [0051]    Mammalian cells are preferred hosts for production of rBPI protein analogs according to the invention because such cells allow for proper secretion, folding, and post-translational modification of expressed proteins. Presently preferred mammalian host cells for production of analogs of the invention include cells of fibroblast and lymphoid origin, such as: CHO-K1 cells (ATCC CCL61); CHO-DG44 cells, a dihydrofolate reductase deficient [DHFR] mutant of CHO Toronto obtained from Dr. Lawrence Chasin, Columbia University; CHO-DXB-11, a DHFR − mutant of CHO-K1 obtained from Dr. Lawrence Chasin; Vero cells (ATCC CRL81); Baby Hamster Kidney (BHK) cells (ATCC CCL10); Sp2/O-Ag14 hybridoma cells (ATCC CRL1581): and NSO myeloma (ECACC No. 85110503).  
         [0052]    Transfection of mammalian cells may be accomplished by a variety of methods. A common approach involves calcium phosphate precipitation of expression vector DNA which is subsequently taken up by host cells. Another common approach, electroporation, causes cells to take up DNA through membrane pores created by the generation of a strong electric field [(Sambrook et al.,  Molecular Cloning, A Laboratory Manual , Cold Spring Laboratory Harbor Press, 16.30-16.31 (1989)]. Selection for transfected cells is facilitated by incorporation in the expression vector of a gene whose product allows the transfected cells to survive and grow under selective conditions. A number of such genes have been identified. These include, among others: (1, neo. a prokaryotic gene which encodes resistance to the aminoglycoside antibiotic G418: (2)  E. coli  guanine phoshporibosyl transferase (gpt), which encodes resistance to mycophenolic acid (MPA) in the presence of xanthine, [Mulligan et al.,  Proc. Nat. Acad. Sci. U.S.A.,  78:2072-2076 (1981)]; (3) dihydrofolate reductase (DHFR). which allows for growth of DHFR −  cells in the absence of nucleosides and gene amplification in the presence of increasing concentration of methotrexate; (4) the hisD gene of  Salmonella trphimurium  which allows growth in the presence of histidinol [Hartman et al.,  Proc. Nat. Acad. Sci. U.S.A.,  85:8047-8051. (1988)]: (5) the trpB gene of  E. coli  [Hartman et al.,  Proc. Nat. Acad. Sci. U.S.A.  85:8047-8051, (1988)], which allows growth in the presence of indole (without tryptophan); and (6) the glutamine synthetase gene, which allows growth in media lacking glutamine. The availability of these selective markers, either alone or in various combinations, provides flexibility in the generation of mammalian cell lines which express recombinant products at high levels. selection of MPA-resistant cells.  
         [0053]    The CHO-K1 cell line is maintained in Ham&#39;s F12 medium plus 10% fetal bovine serum (FBS) supplemented with glutamine/penicillin/streptomycin (Irvine Scientific, Irvine, Calif.). The cells were transfected by electroporation with 40 μg of pING4533 DNA which was first digested with NotI, extracted with phenol-chloroform and ethanol precipitated. Following electroporation, the cells were allowed to recover for 24 hours in non-selective Ham&#39;s F12 medium. The cells were then trypsinized, resuspended at a concentration of 5×10 4  cells/ml in Ham&#39;s F12 medium supplemented with MPA (25 μg/ml) and xanthine (250 μg/ml) and then plated at 10 4  cells/well in 96-well plates. Untransfected CHO-K1 cells are unable to grow in this medium due to the inhibition of pyrimidine synthesis by MPA.  
         [0054]    At 2 weeks, colonies consisting of transfected cells were observed in the 96-well plates. Supernatants from wells containing single colonies were analyzed for the presence of BPI-reactive protein by anti-BPI ELISA using rBPI(1-199) as a standard. In this assay, Immulon-II 96-well plates (Dynatech, Chantilly, Va.) were pre-coated with affinity purified rabbit anti-rBPI(1-199) antiserum. Supernatant samples were added and detection was carried out using affinity purified, biotinylated rabbit anti-rBPI(1-199) antiserum and peroxidase-labeled avidin.  
         [0055]    Approximately 800 colonies were screened in this manner. Thirty-one colonies having the highest production were transferred to 24-well plates for productivity assessment. Cells were grown to confluence in a 24-well plate in Ham&#39;s F12 medium supplemented with 10% FBS. Once the cells reached confluence, the Ham&#39;s F12 medium was removed and 1 ml of HB-CHO serum free medium (Irvine Scientific) plus 40 μl of sterile S-sepharose beads (Pharmacia, Piscataway, N.J.) was added as in co-owned, co-pending U.S. patent application Ser. No. 07/885,501 by Grinna. The cells were then incubated for 7 days after which the S-sepharose beads were removed and washed with 0.1 M NaCl in 10 mM Tris buffer (pH7.5). The product was eluted from the beads by addition of 1.0 M NaCl in Tris buffer and quantitated by ELISA as described above. The top-producing transformant, designated A153, secreted, approximately 3 μg/ml in this assay and was adapted to growth in Excell 301 serum-free medium (JRH Scientific, Lenexa, Kans.). The adapted cells were grown in 1.5 L fermenters in Excell 301 medium in the presence of S-sepharose beads. Productivity was assessed at 120-140 hours by C4 HPLC analysis of product eluted from S-sepharose beads (50 ml aliquots). The productivity was 15-25 μg/L at these stages of the fermentation.  
         [0056]    B. Transfection Of CHO-DG44 Cells With pING4222  
         [0057]    Plasmid pING4222 contains DNA encoding the rBPI(1-193)ala 132  analog fused to the A-MuLv promoter, optimized Kozak initiation sequence, human gamma-1 heavy chain 3′ untranslated region, and the mouse DHFR gene for selection of transfected cells in a nucleoside-free medium.  
         [0058]    The cell line, CHO DG44, was maintained in Ham&#39;s F12 medium plus 10% FBS with glutamine/penicillin/streptomycin. The cells were transfected with linearized pING4222 DNA (40 μg divested with PvuI, phenol-chloroform extracted, ethanol precipitated) using the calcium phosphate method of Wigler, et al.  Cell,  11:223 (1977). Following calcium phosphate treatment, the cells were plated in 96-well plates at approximately 10 4  cells/well and transfectants were obtained by growth in selective medium consisting of αMEM medium lacking nucleosides (Irvine Scientific) and supplemented with dialyzed FBS (100 ml serum dialyzed vs 4 L cold 0.15 M NaCl using 6000-8000 MW cutoff, 16 hours, 4° C.). Untransfected CHO-DG44 cells are unable to grow in this medium due to the DHFR mutation and the lack of nucleosides in the medium supplemented with dialyzed serum.  
         [0059]    At 2 weeks, each well contained approximately 2-3 colonies. The supernatants from wells of a 96-well plate were analyzed for the presence of rBPI(1-193) ala 132  by ELISA as in Section A. Twenty-four highest-producing clones were expanded into 24-well plates in selective αMEM medium supplemented with 0.05 μM methotrexate to induce gene amplification of the rBPI analog-encoding DNA. On observation of growth, cells were transferred to a new 24-well plate and productivity was assessed from S-sepharose eluates as described in section A for the pING4533/CHO-K1 transfectants. The five highest-producing, clones were combined and subcloned by limiting dilution in 96-well plates. The supernatant wells containing single colonies were assayed for levels of rBPI(1-193)ala 132  by ELISA. Twenty highest-producing subclones were next expanded into 24-well plates and subjected to further amplification in the presence of 0.4 μM methotrexate and the levels of product expression for the amplified cells was determined by ELISA. The top producers. Clones 4, 75, and 80. secreted 25-37 μg/ml at 7 days in a 24-well plate containing S-sepharose.  
         [0060]    C. Transfection Of Sp2/O Cells With pING4223 And pING4221  
         [0061]    A strategy adopted in an attempt to achieve optimal expression of desired rBPI products involved transfection of cells having a first expression plasmid with a first marker, screening for the highest producers, and then transfecting the same cells with a second expression plasmid having a different marker. This strategy is described below using Sp2/O cells.  
         [0062]    Plasmid pING4223 contains DNA encoding rBPI(1-193)ala 132  BPI fused to the A-MuLv promoter, optimized Kozak translation initiation sequence, human gamma-1 heavy chain 3′ untranslated sequences, and the gpt marker for selection of MPA-resistant cells.  
         [0063]    The Sp2/O cell line was maintained in DMEM medium supplemented with 10% FBS with glutamine/penicillin/streptomycin. The Sp2/0 cells were transfected by electroporation with 40 μg of pING4223 DNA which had been digested with NotI, extracted with phenol-chloroform and ethanol precipitated. Following electroporation, the cells were allowed to recover for 48 hours in non-selective DMEM medium. The cells were then centrifuged and resuspended at a concentration of 5×10 4  cells/ml in DMEM medium supplemented with MPA (6 μg/ml) and xanthine (250 μg/ml) and plated at 10 4  cells/well in 96-well plates. Untransfected Sp2/O cells are unable to grow in this medium due to the inhibition of pyrimidine synthesis by the MPA. At 1.5-2 weeks, colonies consisting of transfected cells were observed in the 96-well plates. Supernatants from wells containing single colonies were analyzed for the presence of product-reactive protein by ELISA. The highest producers were transferred to a 24-well plate and productivity was assessed in extinct 24-well cultures for cells grown in the presence and absence of 10 −7  M dexamethasone, which causes an increase in expression by the A-MuLv promoter as a result of interactions with the glucocorticoid receptor. The best producer, Clone 2×3, secreted approximately 3 μg/ml and 7 μg/ml in the absence and presence of dexamethasone, respectively.  
         [0064]    Clone 2×3 was next transfected by electroporation with pING4221, which contains the his gene for selection of transfectants. Following recovery for 48 hours in DMEM plus 10% FBS medium, the cells were plated in 96-well plates at approximately 10 4  cells/well in DMEM/FBS supplemented with 6 μg/ml MPA, 250 μg/ml xanthine and 8 mM histidinol. Untransfected cells were unable to grow in the presence of the histidinol and MPA. At 1.5-2 weeks, transfected cells were observed in the 96-well plates. Supernatants from wells containing single colonies were analyzed for the presence of rBPI-reactive protein by ELISA.  
         [0065]    The highest producers were transferred to a 24-well plate. Productivity was assessed as extinct 24-well cultures for cells grown in the presence and absence of 10 −7  M dexamethasone. The best producer, Clone 2×3-130, secreted approximately 15 μg/ml and 30 μg/ml in the absence and presence of dexamethasone, respectively. This isolate was next subcloned by limiting dilution in 96-well plates. Wells containing single colonies were screened by ELISA and the best producers were expanded and retested in 24 well cultures in the presence and absence of 10 −7  M dexamethasone. The highest producing subclone, No. 25, secreted approximately 16 μg/ml and 33 μg/ml in the absence and presence of dexamethasone, respectively.  
         [0066]    D. Transfection Of Sp2/0 Cells With pING4143 And pING4150  
         [0067]    Plasmid pING4143 contains DNA encoding rBPI(1-193)ala 132  fused to the A-MuLv promoter, optimized Kozak translation initiation sequence, and mouse kappa light chain 3′ untranslated sequences along with the gpt gene for selection of MPA-resistant cells. The Sp2/0 cells were transfected by electroporation with 40 μg of pING4143 DNA that was first digested with NotI, phenol-chloroform extracted, and ethanol precipitated. Following electroporation, the cells were allowed to recover for 48 hours in non-selective DMEM medium. The cells were then centrifuged and resuspended at a concentration of 5×10 4  cells/ml in DMEM medium supplemented with MPA (6 μg/ml) and xanthine (250 μg/ml) and plated at approximately 10 4  cells/well in 96-well plates.  
         [0068]    At approximately 2 weeks, colonies consisting of transfected cells were observed in the 96-well plates. Supernatants from wells containing single colonies were analyzed for the presence of BPI-reactive protein by ELISA. The highest producers were transferred to a 24-well plate. Productivity was assessed as extinct 24-well cultures for cells grown in the presence and absence of 10 −7  M dexamethasone. The best producer, Clone 134, secreted approximately 12 μg/ml and approximately 28 μg/ml in the absence and presence of dexamethasone, respectively.  
         [0069]    Clone 134 was transfected by electroporation with the vector, pING4150, which contains DNA encoding rBPI(1-193)ala 132  fused to the A-MuLv promoter and mouse light chain 3′ untranslated region with the his gene for selection of transfectants. Prior to electroporation, the vector was first digested, and phenol-chloroform-extracted and ethanol precipitated. Following recovery for 48 hours in DMEM plus 10% FBS medium, the cells were plated in 96-well plates at approximately 10 4  cells/swell in DMEM/FBS supplemented with 6 μg/ml MPA plus 250 μg/ml xanthine and 8 mM histidinol. Untransfected cells are unable to grow in the presence of MPA and histidinol. At approximately 2 weeks, colonies consisting of transfected cells were observed in the 96-well plates. Supernatants from wells containing single colonies were analyzed for the presence of BPI-reactive protein by ELISA. The highest producers were transferred to a 24-well plate. Productivity was assessed as extinct 24 well cultures for cells grown in the presence and absence of 10 −7  M dexamethasone. The highest producer, Clone 134-11, was re-designated C1770. Clone C1770 secreted 36 μg/ml without dexamethasone and greater than 42 μg/ml in the presence of dexamethasone. This clone (c1770) was deposited with the American Type Culture Collection, 12301 Parklawn Drive, Rockville, Md. 20852 as Accession No. HB 11247.  
         [0070]    E. Transfection Of CHO-K1 Cells With pING4143  
         [0071]    The CHO-K1 cell line was transfected with pING4143 DNA in the manner described in Section A for transfection of CHO-K1 cells with pING4533. At approximately 2 weeks, supernatants from approximately 800 wells containing single colonies were analyzed for the presence of BPI-reactive protein by ELISA. The top producers were transferred to 24-well plates. The top producers, secreting approximately 9-13 μg/ml, may next be adapted to serum-free medium in preparation for growth in fermenters. These may also be re-transfected with a vector, such as pING4150 or pING4154 with his or neo as selective markers, respectively, to provide a cell line which produces even higher levels of rBPI product.  
         [0072]    F. Transfection Of CHO-K1 Cells With pING4144  
         [0073]    Plasmid pING4144 is similar to pING4143 except that it contains the human cytomegalovirus (hCMV) promoter instead of the A-MuLv promoter. The CHO-K1 cell line was transfected with pING4144 DNA in the manner described above in Section A. At approximately 2 weeks, supernatants from approximately 200 wells containing single colonies were analyzed for the presence of BPI-reactive protein by ELISA. The top producers were transferred to 24-well plates and rBPI expression determined in 24-well plates containing sodium butyrate. The top producer (clone 174) secreted approximately 3-5 μg/ml without butyrate and approximately 15-18 μg/ml in the presence of 5 mM butyrate in this assay. This clone, re-designated clone C1771. was deposited with the American Type Culture Collection, 12301 Parklawn Drive. Rockville, Md. 20852 as ATCC accession No. CRL 11246. Top producers may next be adapted to serum-free medium in preparation for growth in fermenters. These may also be re-transfected with a vector, such as pING4151 or pING4155, containing the rBPI gene under control of the hCMV promoter, but with his c −  net) as selective markers, respectively, to provide a cell line which produces even higher levels of BPI.  
         [0074]    G. Transfection Of NSO Cells With pING4143  
         [0075]    NS0 cells were transfected with pING4143 DNA by electroporation. At approximately 3 weeks, colonies consisting of transfected cells were observed in the 96-well plates. Supernatants from wells containing single colonies were analyzed for the presence of BPI-reactive protein by ELISA. The highest producers were transferred to a 24-well plate. Productivity was assessed as extinct 24-well cultures. The highest producers secreted a 15-16 μg/ml. The highest producers may be retransfected with a vector, such as pING4150. as described above to yield even higher producers.  
         [0076]    H. Transfection Of NS0 Cells With pING4232  
         [0077]    NS0 cells were transfected by electroporation with pING4132, which contains DNA encoding rBPI(1-193)ala 132  fused to the optimal Kozak translation initiation sequence cloned into the vector pEE13 [Bebbington, et al.  Biotechnology,  10: 169-175 (1992)]. Vector pEE13 contains the glutamine synthetase gene for selection of transfectants which are able to grow in medium lacking glutamine. At approximately three weeks, colonies consisting of transfected cells were observed in 96-well plates. Supernatants from wells containing single colonies were analyzed by ELISA. The highest producers were transferred to a 24-well plate. Productivity was assessed as extinct 24-well cultures. The highest producers, secreting 7-15 μg in extinct 24-well cultures, may next be subjected to amplification in the presence of various concentrations of methionine sulfoximine.  
         [0078]    I. Transfection Of Sp2/0 Cells with pING4145  
         [0079]    Plasmid pING4145 contains DNA encoding rBPI(1-193)ala 132  fused to the A-MuLv promoter, optimizes Kozak, translation initiation sequence, mouse kappa light chain 3′ untranslated sequences, and a gpt gene for selection of MPA-resistant cells. The Sp2/0 cells were transfected by electroporation with 40 μg of pING4145 DNA that was first digested with NotI, phenol-chloroform extracted, and ethanol precipitated. Following electroporation, the cells were allowed to recover for 48 hours in non-selective DMEM medium, centrifuged, and resuspended at a concentration of 5×10 4  cells/ml in DMEM medium supplemented with MPA (6 μg/ml) and xanthine (250 μg/ml). The cells may then be plated at approximately 10 4  cells/well in 96-well plates. At approximately 2 weeks, colonies consisting of transfected cells are observed in the 96-well plates. Supernatants from wells containing single colonies may then be analyzed for the presence of BPI-reactive protein by ELISA. The highest producers are transferred to a 24-well plate and productivity is assessed as extinct 24-well cultures for cells grown in the presence and absence of 10 −7  M dexamethasone.  
         [0080]    In order to maximize the expression of BPI, the highest producing Sp2/0 transfectant may be transfected by electroporation with a vector which contains gene sequences encoding rBPI(1-193)ala 132  fused to the A-MuLv promoter and mouse light chain 3′ untranslated region with the his gene for selection of transfectants.  
         [0081]    J. Transfection Of CHO-K1 Cells with pING4145  
         [0082]    The CHO-K1 cell line was transfected with pING4145 DNA in the manner described above in Section A. At approximately 2 weeks, supernatants from approximately 500-800 wells containing single colonies may be analyzed for the presence of BPI-reactive protein by ELISA. The top producers are transferred to 24-well plates and BPI expression determined in 24-well plates containing S-sepharose. The top producers are next adapted to serum-free medium in preparation for growth in fermenters. These may also be re-transfected with a vector containing a different selective marker to provide a cell line which produces even higher levels of rBPI product.  
         [0083]    K. Expression of rBPI Products from Insect Cells  
         [0084]    Another eukaryotic system in which rBPI products may be expressed is insect cells which have been infected with a recombinant baculovirus containing DNA encoding an rBPI product. Systems for generating recombinant virus and for achieving expression of recombinant products therefrom are commercially available (Invitrogen, San Diego, Calif.). DNA encoding rBPI(1-199), including the 31 amino acid signal sequence, was cloned into an NheI site in a pBlueBac transfer vector (Invitrogen). Sf9 insect cells (BRL, ATCC CRL 1711) were co-transfected with this vector and with wild type AcMNPV ( Autographa californica  multiple nuclear polyhidrosis virus, Invitrogen). Recombinant viral plaques were then identified, purified, and used to generate high-titer recombinant viral stocks as described in protocols available from BRL.  
         [0085]    The recombinant-produced baculovirus was used to infect further Sf9 cells. To do this, 8 separate 60 mm dishes of Sf9 cells were infected with the baculovirus. Each of the 8 dishes was sampled at different times during the day by collecting medium from a dish of infected cells. Upon collection, the medium was centrifuged at 1000 rpm for 10 minutes and the supernatant was stored at 4° C. Cells were then rinsed once with 4 ml PBS and lysed with 100 μl/dish NP40 lysis buffer (1% NP40, 150 mM NaCl, 50 mM Tris-HCl, pH 8.0) by incubating on ice for 30 minutes. Cells were then collected into an Eppendorf tube with a cell scraper. Cell lysates were then spun in a microfuge for 2 minutes. The lysate supernatant was transferred to a new tube and stored at −20° C. Media samples from each daily time point were analyzed for BPI content by ELISA and lysates were analyzed by Western using an anti-BPI antibody.  
         [0086]    No rBPI product was detectable in the media by ELISA on days 1-4 post-infection. However, on days 5-6 post-infection, a peak of 200-500 ng/ml rBPI product was detected in media samples. Western analysis of the lysates showed a BPI-reactive band of approximately 23 Kd at day 2 post-infection. That band showed increasing intensity through day 6.  
         [0087]    Table II, below, summarizes the transfections detailed in Sections A-J above.  
                           TABLE II                                   Host Cell   Transfected With                           CHO-DG44   pING4222           CHO-K1   pING4533, pING4143,               pING4144, pING4145           NSO   pING4143, pING4232           SP2/O   pING4223 followed by pING4221,               pING4143 followed by pING4150,               pING4145                      
 
       EXAMPLE 3  
     Construction Of Plasmids For in vitro Transcription And Translation Of rBPI (1-199)ala 132  And rBPI (1-199)Ser 135    
       [0088]    In vitro transcription/translation studies were conducted using plasmid pIC127 as a source of DNA encoding rBPI (1-199). Construction of pIC127 was carried out as follows. DNA encoding rBPI (1-199), including the 31-amino acid signal sequence, was PCR amplified from a plasmid containing full-length cDNA encoding BPI in pGEM-72f(+). The amplification was done such that a SalI site was incorporated at the 5′ end and XhoI and SstII sites were incorporated at the 3′ end of the rBPI-encoding sequence by using the primers BPI-3: GTCGACGCATGCGAGAGAACATGGC (SEQ ID NO: 12) and BPI-2: CCGCGGCTCGAGCTATATTTTGGTCAT (SEQ ID NO: 9). The resulting PCR amplified fragment was blunt-end cloned into the SmaI site of the multiple cloning region of plasmid pT7T3 18u (Pharmacia LKB Technology, Piscataway N.J.) in order to generate pIC102.  
         [0089]    The pIC102 insert encoding rBPI (1-199) and the 31-amino acid signal were then excised by digestion of the plasmid with BamHI and Asp718I. A BamHI site flanks the SalI site in pIC102 and an Asp7181 site flanks the SstIII site in pIC102. The ends of the excised fragment were made blunt with T4 DNA polymerase and the blunt fragment was then cloned into plasmid pGEMI (ProMega, Madison, Wis.) which had first been digested with PstI and EcoRI and blunted with T4 DNA polymerase. The resulting construction was designated pIC124 and has the rBPI (1-199)-encodine insert oriented such that its 5′ end is adjacent to the Sp6 promoter in pGEM1.  
         [0090]    The 31-amino acid signal sequence in the pIC124 insert was then excised by removing the region between two HindII sites in pIC124 to create pIC127. The excised region was replaced with a linker which restored the initiation codon (ATG) and the sequence encoding the first amino acid of BPI. Two fragments were isolated from pIC124 digestion with HindII and SstII: (1) the HindII-SstII fragment containing the rBPI (1-199) coding region excluding the codon for the first amino acid; and (2) (he SstII-HindII fragment comprising the remainder of the plasmid. The first codon in the BPI coding sequence and a codon for methionine in front of the BPI sequence were inserted through use of linker formed from two complementary annealed oligonucleotides, BPI-28: GACGCCACCATGGTC (SEQ ID NO: 13) and BPI-29: GACCATGGTGGCGTC (SEQ ID NO: 14). Those two oligonucleotides were ligated together with the HindII-SstII and SstII-HindII fragments from pIC124 to form pIC127.  
         [0091]    Two plasmids, pML101 and pML102, were constructed using pIC127 for in vitro transcription/translation of rBPI(1-199)ala 132  and rBPI(1-199)ser 135 . To do this, pIC127 was digested with SstII and EcoRI and the large SstII-EcoRI fragment was purified. To construct pML101, which contains an rBPI(1-199)ala 132  insert, the EcoRI-SstII fragment from pING4519 was ligated to the SstII-EcoRI fragment from PIC127. To construct pML102, which contains the rBPI (1-199) Ser 135  insert, the EcoRI-sstII fragment from pING4520 was ligated to the sstII-EcoRI fragment from pIC127.  
         [0092]    rBPI(1-199), rBPI(1-199)ser 135 , and BPI(1-199)ala 132  were expressed in vitro from plasmids pIC127, pML101, and pML102 using the TNT SP6 coupled Reticulocyte Lysate System from ProMega (Madison, Wis.). That system allows in vitro coupled transcription and translation of cloned genes using a eukaryotic translation system. Each coupled transcription/translation was carried out using the manufacturer&#39;s protocols with 2 μg of plasmid DNA in a total volume of 25 μl, including  35 S-methionine to generate labeled protein. The labeled protein products were added in 5 μl aliquots to a 20 μl urea sample buffer and heated at 95° C. for 3 minutes. Aliquots (10 μl) of each sample were run on a 15% SDS-Polyacrylamide gel either with or without DTT (50 mM). After fixing and drying the gel, the labeled protein bands were visualized by autoradiography. Results of the autoradiography demonstrate that cDNA encoding rBPI(1-199). rBPI(1-199)ala 132 , and rBPI(1-199)cys 135  expressed protein products of the expected size of approximately 23 Kd for a BPI N-terminal fragment. Moreover, all three expression products, rBPI(1-199), rBPI(1-199)ala 132 , and rBPI(1-199)cys 135 , were capable of generating higher molecular weight species of the size expected for BPI(1-199) dimers, as well as larger species, all of which disappeared upon reduction with DTT. It is thought that the expression of dimeric species in the rBPI(1-199)cys 135  and rBPI(1-199)ala 132  products may be the result of using a cell-free in vitro transcription/translation system. Such a system does not allow proper post-translational processing, folding, etc. which would normally occur in cellular translation. Thus, it may be that proper disulfide linkages do not always form in the in vitro system, leading to formation of dimer in some cases.  
         [0093]    Labeled proteins generated in the above-described in vitro expression system were next tested for LPS binding activity. Wells of microtiter plates were coated with LPS from  Salmonella Minnesota  R7 (Rd mutant) (5 mg/ml in methanol stock culture) in 0.1 M Na 2 CO 3 /20 mM EDTA (ethylenediamine tetraacetic acid) at pH 9.4 (a total of 2 μg LPS in a 50 μl well). Following overnight incubation at 4° C. the wells were rinsed with water and dried at 37° C. The wells were then blocked with 215 μl Dulbecco&#39;s-PBS/0.1% BSA for 3 hours at 37° C. The blocking solution was then discarded and the wells were washed with PBS/0.2% Tween-20. The rBPI samples were then added (2 μl of the translation reactant) to a 50 μl total volume in PBS/0.2% Tween. Following overnight incubation at 4° C., the wells were washed 3 times with PBS/0.2% Tween and the amount of labeled protein remaining in each well was determined by liquid scintillation counting. The results demonstrated that approximately equivalent LPS binding took place for all three BPI species referred to above. rBPI(1-199) displayed binding of 48.690 cpm; rBPI(1-199)ala 132  displayed binding of 59,911 cpm: and rBPI(1-199)cys 135  displayed binding of 52,537 cpm. each of the aforementioned values represents the average of triplicate determinations. The average binding of the control (no DNA) was 5.395 cpm.  
       EXAMPLE 4  
     Product Characterization  
       [0094]    A. Physical Characterization  
         [0095]    Characterization of rBPI products was accomplished using reverse phase (C4) HPLC, cation exchange (MA7C) HPLC, SDS-PAGE, and electrospray ionization mass spectrometry (ESI-NIS). The rBPI products to be characterized were purified from roller bottles or from a 10 Liter fermenter harvest by either a single-step purification procedure or by a multi-step procedure. The single-step procedure was essentially that disclosed in co-pending, co-owned U.S. patent application Ser. No. 07/885.501 by Grinna, incorporated herein by reference, with the addition of a second wash step. In brief, S-sepharose beads were added to a growth medium containing rBPI products. The S-sepharose was then removed from the medium and washed with 20 mM sodium acetate and 100 mM sodium chloride at pH4.0. A second wash was performed with 20 mM sodium acetate and 700 mM sodium chloride at pH4.0. The purified rBPI products were eluted with 20 mM sodium acetate and 1000 mM sodium chloride at pH4.0.  
         [0096]    The multi-step purification procedure involved the purification of pooled batches of rBPI products which had first been purified separately as described above. After purification of each of twenty individual rBPI product batches by the single-step method, the batches were pooled and repurified by first diluting the salt concentration of the pooled batches to 200 mM. The pooled sample was then loaded onto an S-sepharose column and was washed at pH4.0 with 20 mM sodium acetate, and 200 mM sodium chloride followed by 700 mM sodium chloride. The rBPI products were eluted using 20 mM sodium acetate and 1000 mM sodium chloride at pH4.0. The purified rBPI products were then analyzed to determine their physical characteristics.  
         [0097]    1. SDS-PAGE Analysis of rBPI Products  
         [0098]    SDS-PAGE analysis of rBPI products was carried out using 14% polyacrylamide gels and a tris-glycine buffer system under reducing and non-reducing conditions. Protein bands were stained with either Coomassie Blue or silver stain for visualization.  
         [0099]    As shown in FIG. 1, non-reduced rBPI(1-199) appeared as a major band at approximately 23 kD and a minor band at approximately 40 kD. The major band was identified as rBPI(1-199) by comparison with simultaneously-run standards and the minor band was identified as a dimeric form of rBPI(1-199) by immunostaining. Upon addition of a {fraction (1/20)} volume of 0.4 M dithiothreitol (DDT) to a separate sample of rBPI(1-199), SDS-PAGE revealed a single, well-defined band corresponding to the 23 kD monomeric species of rBPI(1-199) identified under non-reducing conditions as described above.  
         [0100]    SDS-PAGE analysis of the rBPI(1-199)ala 132  product revealed a single band which migrated with the single 23 kD rBPI(1-199) band under reducing conditions. Under non-reduced conditions, rBPI(1-199)ala 132  migrated with the faster-migrating of the two closely-spaced bands seen for rBPI(1-199) (corresponding to the 23 kD band). These results, shown in FIG. 2, indicate that rBPI(1-199)ala 132  exists in essentially monomeric form after purification. Thus, rBPI products in which a cysteine residue is replaced by alanine display significant resistance to dimer formation.  
         [0101]    2. Cation Exchange HPLC Analysis of rBPI Products  
         [0102]    Cation exchange HPLC using an MA7C column was also employed to measure the dimer content of rBPI products. A Bio-Rad MA7C cartridge (4.6×30 mm. Bio-Rad Catalog No. 125-00556) equilibrated with 40% buffer B (20 mM MES. 1M NaCl, pH 5.5) at 1.0 ml. min was used. The rBPI(1-199) product was analyzed by diluting a 1 ml sample to 100 μg/ml and 200 μl of the diluted sample was injected onto the column. The rBPI was eluted with a gradient of 40% to 100% buffer B over 6 minutes. Buffer A comprised 20 mM MES at pH5.5. Absorbance was monitored at 229 nm.  
         [0103]    Analysis of rBPI(1-199) revealed two peaks. A first peak eluted with a retention time of approximately 3 minutes as shown in FIG. 3. A second, smaller peak eluted at approximately 6 minutes. The first peak, shown in FIG. 3, represents rBPI(1-199) monomer and the second peak in FIG. 3 represents rBPI(1-199) dimer as determined by comparisons with the retention times of purified monomer and dimer standards. The second (dimer) peak did not appear when samples were reduced with DTT prior to being injected on the column.  
         [0104]    Identical procedures were used to determine the elution pattern of rBPI(1-199)ala 132 . As shown in FIG. 4. rBPI(1-199)ala132 elutes as a single peak with a retention time corresponding to that observed for the rBPI(1-199) monomer peak. There was no evidence of dimer in the rBPI(1-199)ala 132  sample.  
         [0105]    3. Reverse Phase (C4) HPLC and Electrospray-ionization Mass Spectrometry Analysis of rBPI Products  
         [0106]    Microheterogeneity of rBPI products was revealed by reverse phase HPLC and electrospray-ionization mass spectrometry (ESI-MS). For the HPLC analysis, a Brownlee BU-300 C4 column was equilibrated with 37% Mobile Phase B (80% acetonitrile 0.065 TFA) at a flow rate of 0.5 ml/min. Samples (1 ml each of rBPI(1-199) were diluted to 100 μg/ml and 50 μl of the sample was injected. The column was washed with 37% Mobile Phase B for 2.5 minutes and then eluted using a gradient from 35% to 50% Mobile Phase B over 20 minutes. Mobile Phase A was 5% acetonitrile 0.1% TFA and absorbance was monitored at 220 nm.  
         [0107]    The results of reverse phase HPLC analysis of rBPI(1-199) products are shown in FIG. 5. rBPI(1-199) products elute as a second (major) peak with a partially-resolved first minor) peak on the leading edge of the second peak. Upon reduction with DTT only one peak, corresponding to the second peak elutes from the column.  
         [0108]    Identical procedures were used to analyze rBPI(1-199)ala 132  products. As shown in FIG. 6. rBPI(1-199)ala132 eluted as a single peak corresponding to the second (major) peak referred to above.  
         [0109]    The eluates corresponding to the first and second HPLC peaks described above from three separate batches of rBPI(1-199) were isolated and analyzed to determine their content by ESI-MS. Analysis of the eluate which produced the second (major) peak from the rBPI(1-199) run revealed a slightly lower mass than would be expected for a 199-amino acid protein. These data indicate that the most abundant mass found in the second peak eluate corresponded to a 1-193 rBPI protein fragment. However, other species, ranging in size from 1-198 to 1-194. are also present. Analysis of the eluate producing the single peak obtained from HPLC on rBPI(1-199)ala132 revealed results similar to those obtained from the eluate which produced the second (major) peak above. These results are consistent with peptide napping data which reveal truncated carboxy termini in rBPI(1-199) products.  
         [0110]    When the same analysis Was performed on rBPI(1-193) products, significantly reduced C-terminal heterogeneity was observed. The ESI-MS data obtained from rBPI(1-193) products revealed that approximately 85% of the protein contains either the first 191, 193, or 193 (—an N terminal alanine) amino acids of the BPI N-terminal. The results are shown in Table III.  
                                           TABLE III                           Electrospray-Ionization Mass Spectrometry Results       for rBPI(1-193) and rBPI(1-199) HPLC Monomer Peaks                Approximate            Expected   Approximate   Predicted Amino   Relative       rBPI Product   Molecular Mass   Acid Residues   Intensity*               rBPI(1-199)   21407   1-193   50.9%           21606   1-195   28.9%           21505   1-194   20.1%           21738   1-196   &lt;10%               21846   1-197   &lt;10%               21966   1-198   &lt;10%           rBPI(1-193)   21408   1-193   36.2%           21193   1-191   34.1%           21293   1-192   &lt;10%               21477   1-193 + N-   14.5%               terminal alanine           20924   1-189   15.2%                          
 
         [0111]    These data demonstrate that, while the rBPI(1-199)-encoding DNA produced no full-length (i.e. amino acids 1-199 of the BPI N-terminal) protein, the rBPI (1-193)-encoding DNA produced significant amounts of the rBPI(1-193) protein. Based upon these are other ones, it appears that significant reactions in heterogeneity and significant increases in production of the intended protein (i.e. that for which the DNA insert codes may be obtained). while maintaining optimal bactericidal and LPS-binding activity by using truncated forms of the rBPI-encoding DNA. It is expected that truncation of the DNA to be expressed will produce significant reductions in heterogeneity of the expression product to the extent that the DNA to be expressed is not truncated beyond the cysteine at amino acid residue 175. Expression products of truncated forms of DNA encoding rBPI proteins which have in the range of the first 176 amino acids of the BPI N-terminal to the first 193 amino acids of the BPI N-terminal are also expected to retain full bactericidal and LPS-binding activity.  
         [0112]    The ESI-MS data also revealed the presence of microheterogeneity at the amino terminal of rBPI products. Forms of the rBPI product having an alanine residue at the amino terminus were found and confirmed by sequencing of tryptic peptides.  
         [0113]    As shown in FIG. 5, the ESI-MS study of the eluate which produced the first (minor) reverse phase HPLC peak revealed proteins having a mass distribution similar to those which formed the second (major) peak except that each mass value was higher by approximately 119-120 Daltons. These data suggest that the eluate producing the first (minor) HPLC peak described above contains a disulfide-linked cysteine adduct, as this would account for the uniform shift of the mass values.  
         [0114]    To test the hypothesis that the first (minor) reverse phase HPLC peak produced by rBPI(1-199) represents cysteine adducts, rBPI(1-199) was exposed to Ellman&#39;s reagent (dithionitrobenzenoic acid, DTNB) which binds to free sulfhydryl groups in roughly molar equivalents. Such treatment demonstrated that there is less than one mole of free sulfhydryl per mole of rBPI(1-199). Given the presence of three cysteine residues in BPI (at positions 132, 135 and 175). these results support the notion that there is either an intramolecular disulfide link in the rBPI products or that two of the sulfhydryl groups are sterically unavailable. rBPI(1-199)ala 132  showed no reactivity with Ellman&#39;s reagent.  
         [0115]    4. Storage Stability of rBPI(1-199) Products  
         [0116]    Samples of rBPI( 1-199) (1 mg/ml) in a buffer comprising 20 mM sodium citrate. 0.15 M Sodium Chloride buffer. 0.1% poloxamer, and 0.002% polysorbate 80 at pH5.0 were analyzed to determine their storage stability over an 8-week period at the recommended storage temperature of 2-8° C. and at higher temperatures of 22° C. and 37° C.  
         [0117]    The results for storage at 2-8° C. presented in Table IV, show an increase in the presence of dimer (from 1% to 4%), but no significant increase in cysteine adduct or particle formation in the sample.  
                                                   TABLE IV                                       %   %       %   LAL               Storage   Appearance/       Unknown   Dimer   Protein   Cysteine   Inhibition   Particles/   Particles/       Time   Color   pH   Impurities   by HPLC   mg/mL   Adduct   IC 50 ,nG/mL   mL ≧10 μm   mL ≧25 μm               mutual   clear/colorless   5.1   ND   1.0   1.04   12   10   230   5       4 weeks   clear/colorless   5.0   ND   3.2   1.02   11   11   113   2       8 weeks   clear/colorless   5.0   ND   4.4   1.02   14    9   125   5                  
 
         [0118]    However, storage at the increased temperatures of 22° C. and 37° C. show that the presence of dimer and particles in the sample increased dramatically and the amount of cysteine adduct increased moderately. These results are shown in Table V. Additionally, when rBPI(1-199)ala 132  is stored at 22° C. to 37° C. no dimer was detected after storage for two weeks. Under similar conditions, rBPI(1-199) displays significant increases.  
                                                                                                                       TABLE V                                       %                                %   Dimer       %   LAL                   Storage   Appearance/       Unknown   by   Protein   Cysteine   Inhibition   Particles/   Particles/       Temperature   Time   Color   pH   Impurities   HPLC   mg/mL   Adduct   IC 50 ,nG/mL   mL ≧ 10 μm   mL ≧ 25 μm                        mutual   clear/colorless   5.1   ND   1.0   1.04   12   10   230   5       22 C.   4   clear/colorless   5.0   ND   4.5   1.02   12   10   100   4           weeks           8   clear/colorless   5.0   ND   6.8   1.02   14   6   126   3           weeks       37 C.   4   a few particles   5.0   ND   7.9   0.96   16   12   1,709   20           weeks           8   numerous   5.0   ND   13.1   0.88   18   7   20,287   611           weeks   particles                  
 
         [0119]    5. Turbidity of rBPI Product Pharmaceutical Compositions  
         [0120]    Experiments were done to determine the turbidity of various rBPI-containing pharmaceutical compositions. In this context, turbidity refers to the tendency of pharmaceutical compositions to engage in unfolding (i.e., loss of tertiary protein structure) and/or particle formation (interactions between individual proteins to form large (&gt;10 μm) particles). The pharmaceutical compositions tested contained either rBPI(1-199). rBPI(1-199)ala 132  or rBPI(1-193)ala 132  in either a citrate buffer (20 mM sodium citrate 150 mM sodium chloride, pH 5.0) or a citrate buffer containing 0.1% poloxamer 188 (a poloxamer surfactant comprised of polyoxypropylene-polyoxyethylene block copolymer) and 0.002% polysorbate 80 (a polysorbate surfactant comprising polyoxyethylene sorbitan fatty acid ester). As mentioned above, use of a combination poloxamer/polysorbate surfactant system stabilizes pharmaceutical compositions as taught in co-owned, co-pending U.S. patent application Ser. No ______, filed on Feb. 1, 1993 [Attorney Docket No. 27129/31162] by McGregor et al., incorporated herein by reference.  
         [0121]    Samples were analyzed to determine their resistance to turbidity over time at increasing temperature and at either pH 7.0 or pH 5.0. Prior to analysis, all samples were diluted to a concentration of 0.1 mg/ml in either 50 mM potassium phosphate or 20 mM citrate buffer at pH 7.0. Turbidity measurements were obtained by placing samples in quartz cuvettes for use in a Shimadzu UV-160 UV-Vis spectrophotometer (Shimadzu, Pleasanton, Calif.) equipped with a temperature-controlled cuvette holder attached to a recirculating water bath. Upon equilibrating the cuvette holder at the desired temperature (57° C., 65° C., or 85° C. see below), absorbance at 280 nm was measured to confirm that samples had been diluted to the proper concentration. Following this, the absorbance of samples at 350 nm was measured every 2 minutes for 1 hour to determine the change in absorbance over time.  
         [0122]    Results are presented in FIG. 7, wherein “formulated” refers to the rBPI product in citrate buffer containing the poloxamer/polysorbate combination referred to above, and “unformulated” refers to rBPI compounds in citrate buffer alone. A lower rate of change in turbidity (i.e., a lower rate of increase in absorbance over time) indicates increased stability against unfolding and the formation of particles. As shown in FIG. 7, the addition of the aforementioned combination of surfactants resulted in increased stability (resistance to particle formation and unfolding) of all compositions tested. Moreover, the rBPI(1-199)ala 132  and rBPI( 1-193)ala 132  exhibited greatly improved resistance to unfolding and particle formation relative to wild-type compositions—regardless of whether the surfactant combination was present. Similar results were obtained at pH 5.0 and 65° C. at pH 5.0 and 75° C. and at 85° C. respectively.  
         [0123]    Overall, compositions with the surfactant combination and/or the cysteine deletion showed greatly increased stability over time and through increases in temperature as compared to compositions with no surfactant and/or having the wild type BPI(1-199) N-terminal construction.  
         [0124]    B. In Vitro Activity Characterizations  
         [0125]    In Vitro activity of rBPI(1-199)ala 132  products was determined by binding of the products to LPS, by the LAL inhibition assay, and by the bactericidal potency of the products.  
         [0126]    1. Binding Of rBPI(1-199)ala 132  To LPS  
         [0127]    Samples (20 μg to 60 μg each) of  E. coli  (Strain 0111-B4) or  S. minnesota  (Rd mutant) lipopolysaccharide (Sigma Chemical, St. Louis, Mo.) were used to determine the ability rBPI(1-199)ala 132  products to bind LPS.  
         [0128]    The LPS samples were size fractionated by SDS-PAGE and silver stained for visualization or electrotransferred to a nitrocellulose membrane (BA25. Schleicher and Schuell, Keene, N. M.) with appropriate pre-stain standards. The LPS blots were processed by soaking the membrane in 50 mM Tris, 0.2M NaCl (TBS), and 30 mg/ml bovine serum albumin (BSA) at pH 7.4 for 30 minutes at 37° C. Membranes were then incubated in a solution containing 2-4 μg of purified or partially purified rBPI(1-199)ala 132  or a control protein (either rBPI(1-199) or rBPI holoprotein) for 12-18 hours at 21° C. to 42° C. After incubation, the membranes were then washed with TBS-BSA. The solution was changed at least three times over a 30 minute period. The washed membranes were then incubated for 3 hours in a 1:1000 dilution of rabbit anti-rBPI(1-199) in TBS containing 1 mg/ml BSA. Membranes were next washed at least three times and were developed using the Chemiluminescent Detection System (Tropix Systems, Bedford, Mass.) according to the manufacturers instructions, using 5×PBS and 0.25% gelatin (Bio-Rad) in place of 1-block.  
         [0129]    The results, shown in FIG. 1, demonstrate that rBPI(I-199)ala 132  binds to LPS fixed to nitrocellulose as dell or better than rBPI(1-199).  
         [0130]    2.  E. coli  Growth Inhibition Assay  
         [0131]    The  E. coli  broth growth inhibition assay was conducted to determine the bactericidal potency, of rBPI products by treating  E. coli  with rBPI(1-199) or rBPI(1-199)ala 132  analogs and monitoring the inhibition of broth growth as a measure of bactericidal activity. A “rough” strain of  E. coli  with short-chain LPS, designated 15 (a rough UDP-4-epimerase-less mutant of  E. coli  strain 0111:B4), was used in the assay. Cells were grown in a triethanolamine-buffered mineral salts medium (Simon, et. al.  Proc. Nat. Acad. Sci.  51:877 (1964)) which rendered  E. coli  especially sensitive to BPI. The cells were washed and resuspended in 0.9% NaCl to a density of about 5×10 4  cells/ml.  
         [0132]    Approximately 5×10 4  to 10 4    E. coli  cells were incubated for 30-60 minutes with either rBPI(1-199) or with rBPI(1-199)ala 132  analogs at a concentration of 5 μg/ml with a buttered solution (10% Hanks Balanced Salts, 40 mM Tris-HCl, pH 7.5. 0.1% casamino acids) in a volume of 200-400 ml. In addition, the assay was run separately with either rBPI(1-199) or rBPI(1-199)ala 132  analog and 100 mM MgCl 2 . Following incubation, the cells were diluted with 10 volumes of nutrient broth supplemented with 0.9% Nacl. Broth growth was then monitored for several hours.  
         [0133]    The results, shown in FIG. 12, demonstrate that rBPI(1-199)ala 132  analogs possess bactericidal activity as potent or more potent than rBPI(1-199). The bactericidal activity of both rBPI(1-199)ala 132  analogs and that of rBPI(1-199) were reduced, as expected, by MgCl.  
         [0134]    3. LAL Inhibition Assay  
         [0135]    The LAL inhibition assay was used to determine the ability of rBPI(1-193)ala 132  to bind LPS. An LAL inhibition assay is described in Gazzano-Santoro,  Infect. Immun.,  60: 4754-4761 (1992). Results of the LAL assay demonstrate that rBPI(1-193)ala 132  has an IC-50 value of 10, which is equal to that for rBPI(1-199). These data indicate that the analog competes as well as the wild-type rBPI product for binding to LPS.  
         [0136]    C. Efficacy Of rBPI(1-199)ala 132  In An Animal Model Of Lethal Endotoxemia  
         [0137]    An animal model of endotoxemia was used to evaluate the comparative effectiveness of rBPI(1-199)ala 132  and rBPI(1-199) against endotoxic shock.  
         [0138]    Male ICR mice received intravenous injections of 800μg/kg actinomycin-D and either 0.5 μg/kg or 1.0 μg/kg of an endotoxin ( E. coli , Strain 0111:B4). Immediately following the injection of endotoxin, the mice received an intravenous injection (0.5 mg/kg or 5.0 mg/kg) of either rBPI(1-199) or rBPI(1-199)ala 132 . Buffered vehicle was used as a control. Deaths were then recorded over a 7-day period. The results are presented below in Table VI.  
                                                     TABLE VI                                   BPI Dose   # Dead/Total   % Mortality                                        Buffer only   0   14/15    93               0.5 mg/kg   7/15   47           rBPI 23     5.0 mg/kg   8/15   53               0.5 mg/kg   14/15    93           rBPI 23 -cys   5.0 mg/kg   8/16   50                      
 
         [0139]    As seen in Table VI, both rBPI(1-199)ala 132  and rBPI(1-199) provided significant protection against the lethal effects of the endotoxin. Although the present invention has been presented in terms of its preferred embodiments, the skilled artisan realizes that numerous modifications and substitutions are within the scope of the present teaching. For example, substitution of the cysteine at position 132 or 135 of the BPI N-terminal fragment with non-polar amino acids other than alanine or serine is contemplated by the invention. Thus, the scope of the appended claims and any future amendments thereto.   
     
       
       
         1 
         
           
             
14 
 
           
           
             
               1813 base pairs  
               nucleic acid  
               single  
               linear  
             
             
               cDNA  
             
             
               CDS  
                31..1491 

 
             
             
               mat_peptide  
                124..1491 

 
             
              1 

CAGGCCTTGA GGTTTTGGCA GCTCTGGAGG ATG AGA GAG AAC ATG GCC AGG GGC      54 
                                 Met Arg Glu Asn Met Ala Arg Gly 
                                 -31 -30                 -25 

CCT TGC AAC GCG CCG AGA TGG GTG TCC CTG ATG GTG CTC GTC GCC ATA      102 
Pro Cys Asn Ala Pro Arg Trp Val Ser Leu Met Val Leu Val Ala Ile 
            -20                 -15                 -10 

GGC ACC GCC GTG ACA GCG GCC GTC AAC CCT GGC GTC GTG GTC AGG ATC      150 
Gly Thr Ala Val Thr Ala Ala Val Asn Pro Gly Val Val Val Arg Ile 
         -5                   1               5 

TCC CAG AAG GGC CTG GAC TAC GCC AGC CAG CAG GGG ACG GCC GCT CTG      198 
Ser Gln Lys Gly Leu Asp Tyr Ala Ser Gln Gln Gly Thr Ala Ala Leu 
 10                  15                  20                  25 

CAG AAG GAG CTG AAG AGG ATC AAG ATT CCT GAC TAC TCA GAC AGC TTT      246 
Gln Lys Glu Leu Lys Arg Ile Lys Ile Pro Asp Tyr Ser Asp Ser Phe 
                 30                  35                  40 

AAG ATC AAG CAT CTT GGG AAG GGG CAT TAT AGC TTC TAC AGC ATG GAC      294 
Lys Ile Lys His Leu Gly Lys Gly His Tyr Ser Phe Tyr Ser Met Asp 
             45                  50                  55 

ATC CGT GAA TTC CAG CTT CCC AGT TCC CAG ATA AGC ATG GTG CCC AAT      342 
Ile Arg Glu Phe Gln Leu Pro Ser Ser Gln Ile Ser Met Val Pro Asn 
         60                  65                  70 

GTG GGC CTT AAG TTC TCC ATC AGC AAC GCC AAT ATC AAG ATC AGC GGG      390 
Val Gly Leu Lys Phe Ser Ile Ser Asn Ala Asn Ile Lys Ile Ser Gly 
     75                  80                  85 

AAA TGG AAG GCA CAA AAG AGA TTC TTA AAA ATG AGC GGC AAT TTT GAC      438 
Lys Trp Lys Ala Gln Lys Arg Phe Leu Lys Met Ser Gly Asn Phe Asp 
 90                  95                 100                 105 

CTG AGC ATA GAA GGC ATG TCC ATT TCG GCT GAT CTG AAG CTG GGC AGT      486 
Leu Ser Ile Glu Gly Met Ser Ile Ser Ala Asp Leu Lys Leu Gly Ser 
                110                 115                 120 

AAC CCC ACG TCA GGC AAG CCC ACC ATC ACC TGC TCC AGC TGC AGC AGC      534 
Asn Pro Thr Ser Gly Lys Pro Thr Ile Thr Cys Ser Ser Cys Ser Ser 
            125                 130                 135 

CAC ATC AAC AGT GTC CAC GTG CAC ATC TCA AAG AGC AAA GTC GGG TGG      582 
His Ile Asn Ser Val His Val His Ile Ser Lys Ser Lys Val Gly Trp 
        140                 145                 150 

CTG ATC CAA CTC TTC CAC AAA AAA ATT GAG TCT GCG CTT CGA AAC AAG      630 
Leu Ile Gln Leu Phe His Lys Lys Ile Glu Ser Ala Leu Arg Asn Lys 
    155                 160                 165 

ATG AAC AGC CAG GTC TGC GAG AAA GTG ACC AAT TCT GTA TCC TCC AAG      678 
Met Asn Ser Gln Val Cys Glu Lys Val Thr Asn Ser Val Ser Ser Lys 
170                 175                 180                 185 

CTG CAA CCT TAT TTC CAG ACT CTG CCA GTA ATG ACC AAA ATA GAT TCT      726 
Leu Gln Pro Tyr Phe Gln Thr Leu Pro Val Met Thr Lys Ile Asp Ser 
                190                 195                 200 

GTG GCT GGA ATC AAC TAT GGT CTG GTG GCA CCT CCA GCA ACC ACG GCT      774 
Val Ala Gly Ile Asn Tyr Gly Leu Val Ala Pro Pro Ala Thr Thr Ala 
            205                 210                 215 

GAG ACC CTG GAT GTA CAG ATG AAG GGG GAG TTT TAC AGT GAG AAC CAC      822 
Glu Thr Leu Asp Val Gln Met Lys Gly Glu Phe Tyr Ser Glu Asn His 
        220                 225                 230 

CAC AAT CCA CCT CCC TTT GCT CCA CCA GTG ATG GAG TTT CCC GCT GCC      870 
His Asn Pro Pro Pro Phe Ala Pro Pro Val Met Glu Phe Pro Ala Ala 
    235                 240                 245 

CAT GAC CGC ATG GTA TAC CTG GGC CTC TCA GAC TAC TTC TTC AAC ACA      918 
His Asp Arg Met Val Tyr Leu Gly Leu Ser Asp Tyr Phe Phe Asn Thr 
250                 255                 260                 265 

GCC GGG CTT GTA TAC CAA GAG GCT GGG GTC TTG AAG ATG ACC CTT AGA      966 
Ala Gly Leu Val Tyr Gln Glu Ala Gly Val Leu Lys Met Thr Leu Arg 
                270                 275                 280 

GAT GAC ATG ATT CCA AAG GAG TCC AAA TTT CGA CTG ACA ACC AAG TTC     1014 
Asp Asp Met Ile Pro Lys Glu Ser Lys Phe Arg Leu Thr Thr Lys Phe 
            285                 290                 295 

TTT GGA ACC TTC CTA CCT GAG GTG GCC AAG AAG TTT CCC AAC ATG AAG     1062 
Phe Gly Thr Phe Leu Pro Glu Val Ala Lys Lys Phe Pro Asn Met Lys 
        300                 305                 310 

ATA CAG ATC CAT GTC TCA GCC TCC ACC CCG CCA CAC CTG TCT GTG CAG     1110 
Ile Gln Ile His Val Ser Ala Ser Thr Pro Pro His Leu Ser Val Gln 
    315                 320                 325 

CCC ACC GGC CTT ACC TTC TAC CCT GCC GTG GAT GTC CAG GCC TTT GCC     1158 
Pro Thr Gly Leu Thr Phe Tyr Pro Ala Val Asp Val Gln Ala Phe Ala 
330                 335                 340                 345 

GTC CTC CCC AAC TCC TCC CTG GCT TCC CTC TTC CTG ATT GGC ATG CAC     1206 
Val Leu Pro Asn Ser Ser Leu Ala Ser Leu Phe Leu Ile Gly Met His 
                350                 355                 360 

ACA ACT GGT TCC ATG GAG GTC AGC GCC GAG TCC AAC AGG CTT GTT GGA     1254 
Thr Thr Gly Ser Met Glu Val Ser Ala Glu Ser Asn Arg Leu Val Gly 
            365                 370                 375 

GAG CTC AAG CTG GAT AGG CTG CTC CTG GAA CTG AAG CAC TCA AAT ATT     1302 
Glu Leu Lys Leu Asp Arg Leu Leu Leu Glu Leu Lys His Ser Asn Ile 
        380                 385                 390 

GGC CCC TTC CCG GTT GAA TTG CTG CAG GAT ATC ATG AAC TAC ATT GTA     1350 
Gly Pro Phe Pro Val Glu Leu Leu Gln Asp Ile Met Asn Tyr Ile Val 
    395                 400                 405 

CCC ATT CTT GTG CTG CCC AGG GTT AAC GAG AAA CTA CAG AAA GGC TTC     1398 
Pro Ile Leu Val Leu Pro Arg Val Asn Glu Lys Leu Gln Lys Gly Phe 
410                 415                 420                 425 

CCT CTC CCG ACG CCG GCC AGA GTC CAG CTC TAC AAC GTA GTG CTT CAG     1446 
Pro Leu Pro Thr Pro Ala Arg Val Gln Leu Tyr Asn Val Val Leu Gln 
                430                 435                 440 

CCT CAC CAG AAC TTC CTG CTG TTC GGT GCA GAC GTT GTC TAT AAA         1491 
Pro His Gln Asn Phe Leu Leu Phe Gly Ala Asp Val Val Tyr Lys 
            445                 450                 455 

TGAAGGCACC AGGGGTGCCG GGGGCTGTCA GCCGCACCTG TTCCTGATGG GCTGTGGG     1551 

ACCGGCTGCC TTTCCCCAGG GAATCCTCTC CAGATCTTAA CCAAGAGCCC CTTGCAAA     1611 

TCTTCGACTC AGATTCAGAA ATGATCTAAA CACGAGGAAA CATTATTCAT TGGAAAAG     1671 

CATGGTGTGT ATTTTAGGGA TTATGAGCTT CTTTCAAGGG CTAAGGCTGC AGAGATAT     1731 

CCTCCAGGAA TCGTGTTTCA ATTGTAACCA AGAAATTTCC ATTTGTGCTT CATGAAAA     1791 

AACTTCTGGT TTTTTTCATG TG                                            1813 

 
           
           
             
               487 amino acids  
               amino acid  
               linear  
             
             
               protein  
             
              2 

Met Arg Glu Asn Met Ala Arg Gly Pro Cys Asn Ala Pro Arg Trp Val 
-31 -30                 -25                 -20 

Ser Leu Met Val Leu Val Ala Ile Gly Thr Ala Val Thr Ala Ala Val 
-15                 -10                  -5                   1 

Asn Pro Gly Val Val Val Arg Ile Ser Gln Lys Gly Leu Asp Tyr Ala 
              5                  10                  15 

Ser Gln Gln Gly Thr Ala Ala Leu Gln Lys Glu Leu Lys Arg Ile Lys 
         20                  25                  30 

Ile Pro Asp Tyr Ser Asp Ser Phe Lys Ile Lys His Leu Gly Lys Gly 
     35                  40                  45 

His Tyr Ser Phe Tyr Ser Met Asp Ile Arg Glu Phe Gln Leu Pro Ser 
 50                  55                  60                  65 

Ser Gln Ile Ser Met Val Pro Asn Val Gly Leu Lys Phe Ser Ile Ser 
                 70                  75                  80 

Asn Ala Asn Ile Lys Ile Ser Gly Lys Trp Lys Ala Gln Lys Arg Phe 
             85                  90                  95 

Leu Lys Met Ser Gly Asn Phe Asp Leu Ser Ile Glu Gly Met Ser Ile 
        100                 105                 110 

Ser Ala Asp Leu Lys Leu Gly Ser Asn Pro Thr Ser Gly Lys Pro Thr 
    115                 120                 125 

Ile Thr Cys Ser Ser Cys Ser Ser His Ile Asn Ser Val His Val His 
130                 135                 140                 145 

Ile Ser Lys Ser Lys Val Gly Trp Leu Ile Gln Leu Phe His Lys Lys 
                150                 155                 160 

Ile Glu Ser Ala Leu Arg Asn Lys Met Asn Ser Gln Val Cys Glu Lys 
            165                 170                 175 

Val Thr Asn Ser Val Ser Ser Lys Leu Gln Pro Tyr Phe Gln Thr Leu 
        180                 185                 190 

Pro Val Met Thr Lys Ile Asp Ser Val Ala Gly Ile Asn Tyr Gly Leu 
    195                 200                 205 

Val Ala Pro Pro Ala Thr Thr Ala Glu Thr Leu Asp Val Gln Met Lys 
210                 215                 220                 225 

Gly Glu Phe Tyr Ser Glu Asn His His Asn Pro Pro Pro Phe Ala Pro 
                230                 235                 240 

Pro Val Met Glu Phe Pro Ala Ala His Asp Arg Met Val Tyr Leu Gly 
            245                 250                 255 

Leu Ser Asp Tyr Phe Phe Asn Thr Ala Gly Leu Val Tyr Gln Glu Ala 
        260                 265                 270 

Gly Val Leu Lys Met Thr Leu Arg Asp Asp Met Ile Pro Lys Glu Ser 
    275                 280                 285 

Lys Phe Arg Leu Thr Thr Lys Phe Phe Gly Thr Phe Leu Pro Glu Val 
290                 295                 300                 305 

Ala Lys Lys Phe Pro Asn Met Lys Ile Gln Ile His Val Ser Ala Ser 
                310                 315                 320 

Thr Pro Pro His Leu Ser Val Gln Pro Thr Gly Leu Thr Phe Tyr Pro 
            325                 330                 335 

Ala Val Asp Val Gln Ala Phe Ala Val Leu Pro Asn Ser Ser Leu Ala 
        340                 345                 350 

Ser Leu Phe Leu Ile Gly Met His Thr Thr Gly Ser Met Glu Val Ser 
    355                 360                 365 

Ala Glu Ser Asn Arg Leu Val Gly Glu Leu Lys Leu Asp Arg Leu Leu 
370                 375                 380                 385 

Leu Glu Leu Lys His Ser Asn Ile Gly Pro Phe Pro Val Glu Leu Leu 
                390                 395                 400 

Gln Asp Ile Met Asn Tyr Ile Val Pro Ile Leu Val Leu Pro Arg Val 
            405                 410                 415 

Asn Glu Lys Leu Gln Lys Gly Phe Pro Leu Pro Thr Pro Ala Arg Val 
        420                 425                 430 

Gln Leu Tyr Asn Val Val Leu Gln Pro His Gln Asn Phe Leu Leu Phe 
    435                 440                 445 

Gly Ala Asp Val Val Tyr Lys 
450                 455 

 
           
           
             
               25 base pairs  
               nucleic acid  
               single  
               linear  
             
             
               cDNA  
             
              3 

AAGCTTGTCG ACCAGGCCTT GAGGT                                           25 

 
           
           
             
               18 base pairs  
               nucleic acid  
               single  
               linear  
             
             
               cDNA  
             
              4 

CTGGAGGCGG TGATGGTG                                                   18 

 
           
           
             
               19 base pairs  
               nucleic acid  
               single  
               linear  
             
             
               cDNA  
             
              5 

CTCCAGCAGC CACATCAAC                                                  19 

 
           
           
             
               18 base pairs  
               nucleic acid  
               single  
               linear  
             
             
               cDNA  
             
              6 

GAACTTGGTT GTCAGTCG                                                   18 

 
           
           
             
               13 base pairs  
               nucleic acid  
               single  
               linear  
             
             
               cDNA  
             
              7 

GCCACCRCCA TGG                                                        13 

 
           
           
             
               27 base pairs  
               nucleic acid  
               single  
               linear  
             
             
               cDNA  
             
              8 

ACTGTCGACG CCACCATGGC CAGGGGC                                         27 

 
           
           
             
               27 base pairs  
               nucleic acid  
               single  
               linear  
             
             
               cDNA  
             
              9 

CCGCGGCTCG AGCTATATTT TGGTCAT                                         27 

 
           
           
             
               16 base pairs  
               nucleic acid  
               single  
               linear  
             
             
               cDNA  
             
              10 

CTGTAGCTCG AGCCGC                                                     16 

 
           
           
             
               17 base pairs  
               nucleic acid  
               single  
               linear  
             
             
               cDNA  
             
              11 

GGCTCGAGCT ACAGAGT                                                    17 

 
           
           
             
               25 base pairs  
               nucleic acid  
               single  
               linear  
             
             
               cDNA  
             
              12 

GTCGACGCAT GCGAGAGAAC ATGGC                                           25 

 
           
           
             
               15 base pairs  
               nucleic acid  
               single  
               linear  
             
             
               cDNA  
             
              13 

GACGCCACCA TGGTC                                                      15 

 
           
           
             
               15 base pairs  
               nucleic acid  
               single  
               linear  
             
             
               cDNA  
             
              14 

GACCATGGTG GCGTC                                                      15