Abstract:
A biologically pure DNA sequence which encodes an endo 1,4-β-glucanase, useful for the efficient conversion of cellulose to glucose, is disclosed. Also disclosed are recombinant DNA cloning vehicles (vectors) that contain nucleotide sequences that encode for the aforesaid endoglucanase, proteins that exhibit endoglucanase activity, expression-controlling DNA sequences, microorganisms that contain recombinant DNA cloning vehicles, as well as messenger RNA sequences complementary to a DNA strand of the aforesaid DNA nucleotide sequences.

Description:
This is a continuation of U.S. application Ser. No. 07/902,460, filed Jun. 19, 1992, now abandoned, which is a continuation of application Ser. No. 07/630,396 filed Dec. 18, 1990, now abandoned, which is a continuation of U.S. application Ser. No. 06/894,326, filed Aug. 7, 1986, now abandoned. 
    
    
     FIELD OF THE INVENTION 
     This invention is directed to a molecular clone of a gene from the microorganism Cellulomonas fimi and to products derived therefrom. The DNA sequence of this gene encodes for the synthesis of an enzyme, endogluconase, which is useful for the efficient enzymatic conversion of cellulose to glucose. 
     BACKGROUND OF THE INVENTION 
     The efficient conversion of cellulose to a carbohydrate such as glucose which can be used as a starting material for other products, or for the production of food for humans, has been an object of intense research activity for many years. 
     The digestive systems of human beings and many animals cannot break down and absorb nutrient value from cellulose. Only ruminating animals such as cows, which have four stomachs, are capable of breaking down and digesting the complex and highly stable cellulose molecule. Cellulose, if it could be conveniently and economically reduced to a readily human digestible product, would open up a completely new food source for human beings. 
     At the present stage of the biological development of mankind, petroleum hydrocarbons are utilized as starting products for many materials used by humans, for example, polymers such as polyethylene and polystyrene, gasoline for automobiles, and man-made fibres for clothing. Unfortunately, petroleum is a depleting non-renewable resource. Coal can be used as a substitute, but it also is a non-renewable resource. Cellulose, which is the backbone of most flora and occurs naturally on a renewable basis, if it could be efficiently and economically broken down into manageable carbohydrate, could provide a renewable resource which conceivably could replace, at least in part, petroleum or coal as a basic starting block for mankind&#39;s needs. 
     The biological conversion of cellulose to glucose requires the activity of three types of enzymes. The insoluble substrate is attacked first by extracellular cellulases, of which there are two major types: the endo-1,4-β-glucanases (EC 3.2.1.4), or Eng; and the exo-1,4-β-glucanases (cellobiohydrolases, EC3.2.1.91), or exoglucanases (Exg) (Mandels, 1982; Gilbert and Tsao, 1983). The cellobiose resulting from the action of these enzymes is converted to glucose by β-1,4-glucosidases (EC3.2.1.21) or cellobiases (Mandels, 1982; Gilbert and Tsao, 1983). The cellobiases are usually intracellular, but some are extracellular (Mandels, 1982). 
     The inventors have been characterizing the cellulase system of the bacterium, Cellulomonas fimi (Gilkes et al., 1984 a,b; Langsford et al., 1984) by cloning the genes determining all of the components of the system. It is intended to use the cloned genes to characterize the components of the system through nt sequencing and prediction of aa sequences from the nt sequences. Cellulase systems tend to be very complex, and their components can prove difficult to purify by biochemical methods (Mandels, 1982; Gilbert and Tsao, 1983). Gene cloning can serve to identify components when other methods have failed (Gilkes et al., 1984 a,b). The product of a cloned cellulase gene can be produced in a cellulase-free background in an appropriate host microorganism (Whittle et al., 1982; Gilkes et al., 1984 a; Skipper et al., 1985). The individual enzymes then can be used to reconstitute the original cellulase system. Appropriate mixing experiments would help to elucidate the interactions of the components and to define their roles in the degradation of cellulose. 
     SUMMARY OF THE INVENTION 
     This invention is directed to cloned C. fimi DNA fragments expressing Eng activities, the characterization and structure of the cenA gene, and an analysis of functional regions of the protein. 
     The DNA sequence in Cellulomonas fimi which encodes an endo 1,4-β-glucanase EC3.2.1.4 (endoglucanase) has been cloned and determined. The total amino acid sequence of the endoglucanase has been determined from the DNA sequence, and a partial sequence confirming this has been determined directly by analysing the purified protein. The gene directs the synthesis of an enzyme which is necessary for the efficient enzymatic conversion of cellulose to glucose. 
     A derivative of the cloned gene on plasmid pcEC-2 in Escherichia coli C600 has been deposited at American Type Culture Collection, Rockville, Md., U.S.A., under ATCC No. 67101. 
     It is known that the enzymatic process developed for the conversion of cellulose to glucose will require endoglucanase as an essential component. Isolation of the gene and determination of its sequence thus facilitates development of such a process. The sequence of the gene can be manipulated to improve the characteristics of the enzyme, e.g., increasing the activity of the enzyme to increase the rate of conversion of cellulose to glucose, or by increasing the rate of production of the enzyme so that more cellulose can be degraded. Similarly, the stability of the enzyme to pH and temperature can be improved by altering the sequence of the gene. 
     In one aspect, the present invention is directed to a biologically pure plasmid having therein a DNA sequence with encodes an endo 1,4-β-glucanase (endoglucanase) which is useful for the efficient conversion of cellulose to glucose. 
     In another aspect, this invention is directed to an isolated cenA gene which is useful for synthesizing an endoglucanase enzyme which hydrolyses β-1,4 glycosidic linkages in the interior of a cellulose molecule. 
    
    
     DRAWINGS 
     In the drawings: 
     FIGS. 1a through 1d represents a diagram of plasmid pEC2 and its deletion derivatives pEC2.1, pEC2.2 and pEC2.3. The circular plasmids are shown in a linear fashion for clarity of comparison; 
     FIG. 2 depicts the immunoprecipitation of polypeptides encoded by pEC2 and its deletion derivatives, pEC2.1, pEC2.2 and pEC2.3; 
     FIG. 3(a) represents the hybridization results of the DNA&#39;s restricted with an AvaII probe; 
     FIG. 3(b) represents a restriction map of a SmaI fragment derived from pcEC2. 
     FIGS. 4a through 4c represents a sequence flow-chart of the protocol used for producing and screening deletions; and, 
     FIGS. 5A through 5F represents the nucleotide sequence of the nucleic acid (the cenA gene) and the amino acid sequence of the Endoglucanase protein, deduced from the gene. 
    
    
     DETAILED DESCRIPTION OF THE INVENTION 
     DEFINITIONS 
     The following abbreviations and symbols are used in the specifications and claims. 
     
         ______________________________________aa            amino acid(s)Ap            ampicillinBamHI         a prototypic restriction enzyme         which recognizes the nucleotide         sequence G GATCCbp            base pair(s)cDNA          complementary DNACMC           carboxymethylcelluloseCMCase        carboxymethylcellulasecenA          gene coding for EngDNA           deoxyribonucleic acidEng           endoglucanase(s)Exg           exoglucanase(s)ExoIII        exonuclease IIIGenome        entire complement of genetic         material in a chromosome setIPTG          isoporopyl- -D-thiogalactopyr-         anosidekb            1000 bpKDal          kilodalton(s)M.sub.r       apparent relative molecular         massmRNA          messenger RNAnt            nucleotide(s)ONPG          o-nitrophenyl- -D-galactosidePalindrome    a sequence of DNA that is the         same when opposite strands are         read in the same direction (eg.         5&#39; to 3&#39;)Plasmid       autonomous self-replicating         extra chromosomal circular DNAPolIk         Klenow (large) fragment of         E. coli DNA polymerase IPromoter      region of DNA involved in binding         of RNA polymerase to initiate         transcriptionR             resistantReplication   DNA synthesisReplicon      the unit which controls         individual acts of replication;         it has an origin at which         replication is initiated and it         may have a terminus at which         replication stopsRF            replicative formRNA           ribonucleic acidrRNA          ribosomal RNAS             sensitiveSDS           sodium dodecyl sulfateTc            tetracyclineTranscription synthesis of RNA using a DNA         templateTranslation   synthesis of protein on a mRNA         templateu             unit(s)Vector        a plasmid or phage into which a         foreign DNA may be inserted to be         clonedXGal          5-bromo-4-chloro-3-indolyl-β-D-         galactopyranoside______________________________________ 
    
     The term &#34;corresponds&#34; in its various grammatical forms is used herein and in the claims in relation to nucleotide sequences to mean the nucleotide sequence described containing only conservative codon substitutions that encode for particular amino acid residues along the protein sequence. 
     The term &#34;conservative codon substitution&#34; as used above is meant to denote that one codon has been replaced by another leading to translation of a protein in which an amino acid residue has been replaced by another, biologically similar residue. Examples of conservative substitutions at the amino acid residue (translation) level include the substitution of one hydrophobic residue such as Ile, Val, Leu or Met for another, or the substitution of one polar residue for another such as between Arg and Lys, between Glu and Asp or between Gln and Asn, and the like. 
     In some instances, the replacement of an ionic residue by an oppositely charged ionic residue such as Asp by Lys has been termed conservative in the art in that those ionic groups are thought to merely provide solubility assistance. In general, however, replacement of an ionic residue by another ionic residue of opposite charge is considered herein to be &#34;radical replacement&#34;, as are replacements between nonionic and ionic residues, and bulky residues such as Phe, Tyr or Trp and less bulky residues such as Gly, Ile and Val. 
     The terms &#34;nonionic&#34; and &#34;ionic&#34; residues are used herein in their usual sense to designate those amino acid residues that normally either bear no charge or normally bear a charge, respectively, at physiological pH values. Exemplary nonionic residues include Thr and Gln, while exemplary ionic residues include Arg and Asp. 
     At the nucleotide level, the term &#34;corresponds&#34; is also meant to denote that a nucleotide of a codon can be replaced by another nucleotide so that the codon containing the conservative substitution encodes for the same amino residue as did the unsubstituted codon. Such redundancy of different codons being translated to the same amino acid residue is well known in the art, as elsewhere discussed herein. 
     The term &#34;biologically pure&#34; as used herein refers to a biological substance free from all heterogeneous or extraneous matter. 
     When used in a context describing or depicting nucleotide sequences, the purine or pyrimidine bases forming the nucleotide sequences are depicted as follows: 
     A--deoxyadenyl 
     G--deoxyguanyl 
     C--deoxycytosyl 
     T--thymidyl 
     In describing a nucleotide sequence each three-letter triplet constituted by the bases identified above represents a trinucleotide of DNA (a codon) having a 5&#39;-end on the left and a 3&#39;-end on the right. 
     The amino acid sequences of the proteins described herein and defined by the claims are depicted by their three-letter or single-letter symbols that are identified and correlated in below: 
     
         ______________________________________SYMBOLS FOR AMINO ACIDS       Three-Letter                Single-Letter______________________________________Alanine       Ala        AArginine      Arg        RAsparagine    Asn        NAspartic acid Asp        DCysteine      Cys        CGlutamic acid Glu        EGlutamine     Gln        QGlycine       Gly        GHistidine     His        HIsoleucine    Ile        ILeucine       Leu        LLysine        Lys        KMethionine    Met        MPhenylalanine Phe        FProline       Pro        PSerine        Ser        SThreonine     Thr        TTryptophan    Trp        WTyrosine      Tyr        YValine        Val        V______________________________________ 
    
     Full citations of the scientific publications referenced throughout the specification are provided in a References section herein below. Amino acid residues of proteins and polypeptides are in their natural, L, configurations. 
     GENERAL 
     Two BamHI fragments (0.8 and 5.2 kb) of Cellulomonas fimi containing an endoglucanase (Eng) gene (cenA) were individually cloned into the BamHI site of pBR322. They were found to express carboxymethylcellulase activity in Escherichia coli. The nucleotide (nt) sequence of the cenA gene was determined by sequencing overlapping deletions. The cenA gene has been found to be 1350 bp long encoding a polypeptide of 449 amino acids (aa) and a stop codon. The 0.8-kb BamHI component encodes the first 76 aa, whereas the 5.2-kb BamHI component encodes the rest of the Endoglucanase (Eng). The Eng lacking the N-terminal 76 aa retains its activity and antigenicity, and it forms an active fusion protein with the N-terminal portion of the Tc R  determinant. The C-terminal region of the Eng is crucial for activity and deletion of as little as 12 aa from that end has been found to result in the loss of all Eng activity. The N-terminal 31 aa of the Eng constitute a leader peptide which appears to be functional in exporting the enzyme to the periplasm in E. coli. 
     MATERIALS USED AND GENERAL METHODS FOLLOWED 
     (a) Bacterial Strains, Media and Vectors 
     Except for E. coli JM101, the bacterial strains and the media used for their cultivation have been known and described previously (Whittle et al., 1982; Gilkes et al., 1984a). E. coli JM101 was the host for the M13 phage vectors (Messing, 1979; Yanisch-Perron et al., 1985). The plasmids pBR322 (Bolivar et al., 1977), pEC2 (Gilkes et al., 1984a) and phage M13mp18 (Yanisch-Perron et al., 1985) have been described previously. 
     (b) Enzyme Assays and Identification of Plasmid-coded Proteins 
     Cellulase activity in the total cell extracts prepared by the French press procedure (Whittle et al., 1982) was measured colorimetrically using CMC as substrate (Miller et al., 1960). One unit of enzyme released 1 umol of glucose equivalents per min, as determined by reference to a standard curve. Plasmid-encoded proteins were identified in maxicells (Sancar et al., 1979) after immunoprecipitation (Ivarie and Jones, 1979; Gilkes et al., 1984a). 
     (c) DNA Isolation and Fractionation 
     The isolation of chromosomal DNA from C. Fimi has been described previously (Whittle et al., 1982). Plasmid DNA for restriction analysis was isolated by the alkaline lysis procedure (Maniatis et al., 1982). Plasmid DNA to be sequenced was purified by banding in CsCl-ethidium bromide density gradients (Manjarls et al., 1982). The M13 RF and viral DNAs were isolated from infected cultures (Messing, 1983). DNA restriction fragments were resolved by agarose gel electrophoresis (Maniatis et al., 1982). 
     (d) Enzymes and Reagents 
     All restriction endonucleases were purchased from Bethesda Research Labs or PL Biochemicals; and were used as recommended by the suppliers. T4 DNA ligase, SI nuclease, ExoIII, PolIk, and T4 DNA polymerase were purchased from PL Biochemicals. Calf intestinal phosphatase was obtained from Boehringer-Mannheim. IPTG, Xgal and ONPG were obtained from Sigma. Nitrocefin was received from Glaxo Group Res. Ltd., Greenford, England. Radioactive deoxyribonucleoside 5&#39;-triphosphates and  35  S-methionine were obtained from NEN. 
     SPECIFIC PROCEDURES AND RESULTS OBTAINED 
     (a) The Localization of the cenA Gene in pEC2 
     The original library of C. fimi genes was constructed by ligating a BamHI digest of genomic DNA into the BamHI site of pBR322. E. coli was transformed with the plasmid mixture. Ap R , Tc S  clones were screened for expression of C. fimi cellulases with antibody prepared against proteins secreted by C. fimi during growth on cellulose. Positive clones were characterized further by determination of enzymatic activities (Whittle et al., 1982; Gilkes et al., 1984a). The clone, pEC2, was shown to encode an Eng (Gilkes et al., 1984b) on an insert of about 5.2 kb (Gilkes et al., 1984a). The gene was localized within the insert by deleting portions of the insert using the restriction endonucleases AvaI and PvuII (see FIG. 1). 
     FIG. 1 represents a diagram of the plasmid pEC2 and its deletion derivatives pEC2, pEC2.1, pEC2.2 and pEC2.3. The circular plasmids are shown in a linear fashion for the clarity of comparison. (a) pEC2; (b) pEC2.1; (c) pEC2.2; and (d) pEC2.3. The open bar represents pBR322 DNA. The solid bar represents C. fimi DNA. The dashed lines represent the regions deleted in each derivative. The total length of each plasmid is indicated; the C. fimi inserts are 5.2 kb in (a); 1.9 kb in (b); 2.4 kb in (c); and, 3.5 kb in (d). The deletions in (b) and (d) extend to the AvaI site (A) and the PvuII site (Pv) of pBR322, respectively. However, the PuvII site was not regenerated in (d) after religation. The deletion in (c) was confined within the two SmaI or AvaI sites (S/A) of the insert. The numbers 1 to 7 represent the restriction fragments obtained by digesting (a) with BamHI+SmaI. Restriction enzymes are: A, AvaI; b, BamHI; Bg, BglII; E, EcoRI; H, HindIII; K, KpnI; p, PstI; Pv, PvuII; R, EcoRV; and S, SmaI. 
     The shortest, uninterrupted fragment of the 5.2-kb insert which expressed CMCase activity equal to that of pEC2 was 1.4-kb long; it was found in pEC2.2 (see FIG. 1c; Table I below). Two other subclones expressed as much CMCase activity as pEC2. These were pEC2.1 and pEC2.3 (see FIGS. 1b and d; Table I below). All three clones shared the lefthand 1.4-kb fragment of the 5.2-kb insert. It was concluded that the Eng coding sequence was contained within this 1.4-kb fragment. 
     (b) The Eng Expressed as a Fusion Protein in E. coli 
     All of the deletion mutants described in FIG. 1 were found to encode an immunoprecipitable polypeptide of 53 kDa (see FIG. 2). 
     FIG. 2 illustrates the immunoprecipitation of polypeptides encoded by pEC2 and its deletion derivatives. It was found that E. coli CSR603 was transformed with either pEC2, pEC2.1, pEC2.2, or pEC2.3. The proteins encoded by each plasmid were labelled according to the maxicell procedures of Sancar et al. (1979). The labelled proteins were then precipitated with antibodies against the Eng, and the precipitates were analysed by SDS-polyacrylamide gel electrophoresis as described previously (Gilkes et al., 1984a). Four sets of protein samples are shown, and each set is derived from one of the four plasmids as indicated. Lanes 1, the labelled proteins before treatment with antisera; lanes 2, the protein precipitated with a monoclonal antibody A2/23.11.32 (Langsford et al., 1984) directed against C. fimi cellulase; lanes 3, protein precipitated with antisera raised against CMC-induced C. fimi extracellular enzymes (Whittle et al., 1982). The open triangle indicates the immunoprecipitated protein in lanes 2 and lanes 3 of all four samples. Close triangles represent M r  markers; and numbers refer to sizes (kDa). 
     Since all of the deletion mutants described in FIG. 1 encoded an immuno-precipitable polypeptide of 53 kDa (FIG. 2), it was concluded that the sequence encoding CMCase activity and antigenicity lies within the 1.4-kb fragment of C. fimi DNA common to the four plasmids. However, a fragment of 1.4 kb is not quite sufficient to encode a 53-kDa polypeptide. This suggested that the CMCase activity determined by the plasmids was a fusion polypeptide containing a fragment of the Tc R  determinant and the Eng. In this case, the cenA gene would lack the C. fimi transcriptional and translational signals controlling the expression of the gene and a portion of the N-terminal coding sequence. This was supported by the fact that either inverting the C. fimi insert with respect to the Tc R  promoter (Stuber and Bujard, 1981) or deleting the Tc R  promoter resulted in a drastic reduction of cellulase expression from the respective constructs (see Table I; pEC2.2i, pEC2.1 HB). In addition, frameshift mutations introduced into the Tc R  coding portion of the proposed fusion protein led to a loss of CMCase activity (see Table I; pEC2.1 Ks, pEC2.1 RB). 
     (c) Cloning of the N-Terminus of the cenA Gene 
     In order to clone the N-terminus of the cenA gene, a partial BamHI digest of C. fimi DNA was ligated into the BamHI site of pBR322. Clones were screened by the CMC plate assay (Teather and Wood, 1982). The plasmids from CMCase-producing clones were digested to completion with BamHI. A plasmid, pcEC2, was obtained that contained the 5.2-kb fragment of pEC2 (FIG. 1a) and an additional 0.8-kb fragment 5&#39; to the region known to code for CMCase activity. The 0.8-kb and 5.2-kb fragments were shown to be contiguous on the C. fimi genome by Southern hybridization analysis (see FIG. 3). 
     FIG. 3 represents evidence that the 0.8-kb fragment and the C. fimi insert of pEC2 are contiguous on the C. fimi genome. C. fimi genomic DNA was cleaved to completion by SmaI. The DNA was then digested with either MluI, XhoI, PvuII, or BamHI. The cleaved DNAs were fractionated by 1.2% agarose gel electrophoresis, and hybridized with a  32  P-labelled AvaII probe according to the procedures of Southern (1975). The AvaII probe was obtained from the 0.8-kb fragment (as shown in b), and was labelled with [- 32  p]dATP,--dGTP, and --dCTP by PolIk. FIG. 3(a) depicts the hybridization results of the restricted DNAs with the AvaII probe. Lane 1: pcEC2 digested with SmaI (positive control). Lane 2-6: C. fimi DNA digested with SmaI (lane 2), SmaI+MluI (3), SmaI+XhoI (4), SmaI+PvuII (5), and with SmaI+BamHi (6). The arrows indicate the hybridized bands that would be expected from the restriction map of pcEC2. The numbers indicate the positions of the smaller size markers (in kb) of DNA digested with EcoRI+HinIII. FIG. 3(b) presents a restriction map of the SmaI fragment derived from pcEC2. The hatched bar represents the 0.8-kb portion; the open bar represents the portion from pEC2&#39;s insert; the solid bar represents the AvaII probe. The numbers are the coordinates in bp. Restriction enzymes are: B, BamHI; M, MluI; Pv, PvuII; S, SmaI; and X, XhoI. 
     The 0.8-kb BamHI fragment from pcEC2 was purified and ligated into BamHI-digested pEC2.1 (FIG. 1b). When the fragment was inserted in the same orientation as in pcEC2, this plasmid, designated pcEC2.1, gave the same level of CMCase activity as pcEC2 (Table I). However, when the fragment was inserted in the opposite orientation, this plasmid, designated pciEC2.1, gave very little CMCase activity (Table I below). This suggested first that the 0.8-kb fragment contained a translation initiation signal and second that the entire Eng-coding sequence lay within the 2.2 kb comprising the 0.8-kb fragment and the first 1.4 kb of the 5.2-kb fragment of C. fimi DNA. 
     (d) The Sequence of the cenA Gene 
     The BamHI fragment in pEC2.2 (FIG. 1c) was 2.4-kb long, and it contained the 1.4 kb to the right of the junction. The fragment was subcloned into M13mp18, and a series of unidirectional, overlapping deletions was generated in it with ExoIII (Henikoof, 1984; see legend to FIG. 5 below). This approach allowed the sequencing of the left-hand part of the fragment preferentially, because the time of digestion with ExoIII could be adjusted to give a series of deletions of approximately the required length. 
     A novel procedure was used to generate deletions for use in sequencing the 0.8-kb BamHI fragment from pcEC2. The procedure allowed the isolation in a simple screening of a set of six overlapping sequences, three for each complementary strand, which covered the entire fragment (see FIG. 4). 
     FIG. 4 represents a flowsheet of the protocol for production and screening of deletions. Specifically, the following protocol was used for producing and screening deletions created by SalI cleavage of the 0.8-kb fragment from pcEC2. (A) The 0.8-kb BamHI fragment (open bar; arrows indicate direction of transcription) was cloned into the EcoRI site of M13mp18 (m.c.s. represents the multiple-cloning sites). Two recombinant DNA products, pWT and pF, carried the 0.8-kb fragment in opposite orientations; they were screened by restriction analysis of RF molecules. (B) The RF DNA from each phage type was cleaved with SalI, diluted, and religated. (C) The deletion mutants were identified by a rapid phage hybridization test (C test; Messing, 1983). Each unknown phage of the class p SaWT was annealed with an unknown phage of the class p SaF. Those which did not anneal were then annealed with pF and pWT, respectively. Those which annealed were sequenced (see FIG. 5). The same procedure was used to generate SmaI (S) deletions for sequencing. Restriction enzymes are: B, BamHI; E. EcoRI; H, HindIII; S. SmaI; and Sa, SalI. 
     The sequence corresponding to the cenA gene was located and its reading frame was established by matching the aa sequences predicted by the nt sequence with the sequence of the first 31 aa at the N-terminus of the Eng purified from C. fimi (FIG. 5). The nt sequence determining these 31 aa falls entirely within the 0.8-kb fragment of pcEC2. A putative start codon (ATG) occurs 93 nt upstream from the first nt of the codon defining the N-terminal alanine of the mature Eng. The first stop codon in frame with this ATG is a TGA 1347 nt downstream from the A of ATG. This means that the primary translation product of the cenA gene is 449 aa long, and that the first 31 aa at the N-terminus are removed to generate the mature Eng of 418 aa. The predicted aa composition of the mature enzyme agrees closely with that determined for the enzyme purified from C. fimi. The predicted sequence gives a protein with an M r  of 51,837. The enzyme as purified from E. coli has an apparent M r  of 51,837. The enzyme as purified from C. fimi has an apparent m R  of 58,000; however, this form of the enzyme is glycosylated (Gilkes et al., 1984; Langsford et al., 1984). 
     (e) Transcriptional and Translational Signals for the cenA Gene 
     FIG. 5 illustrates the nt sequence of the cenA gene and the deduced aa sequence of the Eng protein. The strategy of generating unidirectional overlapping deletions of the 2.4-kb BamHI insert of pEC2.2 is essentially the same as described (Henikoff, 1984) except for the following changes. The BamHI insert was blunt ended with PolIk and was ligated in both orientations with EcoRI cleaved M13mp18 (sticky ends filled in by PolIk). 5 ug of the recombinant RF DNA (of each orientation) were used as the starting material. The DNA was cleaved completely with BamHI to give an ExoIII susceptible end and with PstI to produce an ExoIII resistant end. The conditions used for the ExoIII treatment were as described previously except that 12 aliquots of treated DNA were removed successively at intervals of 30 min. The ExoIII reaction was stopped, and aliquots of DNA were treated successively with S1 nuclease, PolIk and DNA ligase. 20 ul of each ligated sample was used to transfect E. coli JM101 cells by standard procedures (Messing, 1983). RF DNA was prepared from individual plaques (Messing, 1983) and analyzed using restriction endonucleases. Clones containing DNA of appropriate insert size were chosen for the sequencing. Sequencing of the overlapping deletion fragments from the two BamHI fragments was performed by the dideoxy termination method (Sanger et al., 1977). The coding region (set in triplets) starts at +1 (A of ATG) and ends at +1347. the last digit of each number is aligned with the numbered nt. A Shine-Dalgarno (S. D.) type sequence before the ATG start codon is underlined. The downward arrow indicates the leader sequence processing site. The underlined aa residues were determined by automated Edman degradation of the purified native Eng. The BamHI site between the 0.8-kb fragment and the insert of pEC2 is boxed. A prominent (pro-thr) 4  -thr-(pro-thr) 7  aa sequence is overlined. 
     As can be seen in FIG. 5, the TGA stop codon is followed closely by a perfect 16-bp palindrome which could be a transcriptional termination signal. The 16-bp palindromic sequence following the stop codon is indicated by the inverted arrows. The sequence preceding the ATG start codon contains a potential ribosome-binding site (Shine and Dalgarno, 1974; FIG. 5), but it does not contain a sequence resembling other prokaryotic promoter sequences (Moran et al., 1982; Hawley and McClure, 1983). However, S1 mapping indicated a potential transcriptional start point 46 nt upstream from the start codon. The expression of the gene in E. coli depends on the Tc R  promoter. When the Tc R  promoter (Stuber and Bujard, 1981) was removed from pcEC2.1, the level of expression of the cenA gene was reduced by 94% (Table I, pcEC2.1 HB). This suggests that the presumed promoter from C. fimi was not functional in E. coli. 
     (f) Functional Regions of the Eng 
     The expression of the cenA gene fragment in pEC2 and its derivatives as an active fusion polypeptide shows that the N-terminal fragment of the native enzyme is not essential for the enzyme activity. It remains to be determined if its absence affects the kinetics or substrate binding of the enzyme. It is possible that the N-terminus of the Tc R  determinant substitutes to a degree for the missing segment of the enzyme. 
     Deletion of DNA coding for the last 12 aa from the C-terminal end of the cenA gene (FIG. 5) by ExoIII digestion resulted in the loss of all Eng activity (data not shown). This demonstrates that the C-terminus of the Eng is essential for activity. However, it is not yet clear if these aa are directly or indirectly involved in active site function. 
     (g) The Signal Peptide of the Eng 
     The nt sequence of the cenA gene predicts an initial sequence of 31 aa having many of the features of protein signal sequences such as charged aa at the N-terminus, lengthy hydrophobic sequence, and a gln-ala-ala processing site (Inouye and Halegoua, 1980; Kreil, 1981; Watson, 1984; Wickner and Lodish, 1985). This sequence appears to function in the export of the Eng to the periplasm in E. coli. More than 50% of the CMCase activity determined by pcEC2 is found in the periplasm (Table II below). This contrasts with the cellular location of the polypeptide determined by pEC2. The Eng leader sequence is missing in this plasmid, and only 15% of the CMCase activity it determines is found in the periplasm (Table II). This latter &#34;Eng&#34; is a hybrid protein, with the N-terminus of the Tc R  determinant of pBR322 replacing the first 76 aa of the pre-Eng. The Tc R  determinant is an integral membrane protein (Sutcliffe, 1979; Nguyen et al., 1983), which implies that its N-terminus has features which lead to the incorporation of the Tc R  protein into the membrane (Kreil, 1981; Nguyen et al., 1983; Wickner and Lodish, 1985). However, the Tc R  N-terminus does not operate as efficiently for secretion of the Eng as does the signal peptide of the Eng itself. 
     (h) The pro-thr Sequence of the Eng 
     The predicted aa sequence of the mature Eng contains a very striking feature. The aa 143-165 corresponding to nucleotides 426-495, respectively are either threonine or proline (see FIG. 5). The sequence of these residues corresponds very closely with a sequence containing only proline and threonine which occurs in the predicted aa sequence of an Exg from C. fimi (O&#39;Neill et al., 1986). The function of this conserved sequence remains to be determined. 
     
                                           TABLE I__________________________________________________________________________This Table tabulates the Eng activities of various cenA clones              CMCase specificClone  Description activity.sup.a                       Ref.__________________________________________________________________________pEC2   parental clone              0.215.sup.b                       FIG. 1aPEC2.1 Eng.sup.+ deletion              0.279    FIG. 1bpEC2.2 derivatives of pEC2              0.259    FIG. 1cpEC2.3             0.232    FIG. 1dpEC2.2i  derivatives of pEC2              0.00077  c  produced to investigatepEC2.1 HB  transcription              0.00056  dpEC2.1Ks  derivatives of pEC2              0.0059   e  produced to investigatepEC2.1 RB  translation 0.0056   fpcEC2  pEc2 plasmid with the              0.0152   RESULTS AND  0.8-kb fragment at the                       DISCUSSION  insert&#39;s 5&#39; end      Section cpcEc2.1  products of functional              0.0150   RESULTS AND  investigation of the DISCUSSIONpciEC2.1  0.8-kb fragment              0.00047  Section cpcEC2.1 HB  derivative of pcEC2.1              0.00090  g  with the Tc.sup.R promoter  deleted__________________________________________________________________________ LEGEND .sup.a Specific activity is expressed as U/mg of protein, where U is umol of glucose equivalents released per min. .sup.b From Gilkes et al. (1984 a,b). .sup.c Obtained by inverting the BamHI insert of pEC2.2. .sup.d Obtained by deleting the small HindIIIBamHI fragment containing th Tc.sup.R promoter (Stuber and Bujard, 1981) from pEC2.1.) .sup.e Obtained by linearizing pEC2.1 with BamHI, filing in the cohesive ends with PolIK, and ligating the resulting blunt ends. .sup.f Obtained by deleting the smaller EcoRVBamHI fragment from pEC2.1. .sup.g Obtained by deleting the smaller HindIIIBamHI fragment from pcEC2.1. 
    
     
                       TABLE II______________________________________This Table tabulates the distribution of enzyme activities indifferent cellular locations of clones pEC2 and pcEC2        Enzyme activity.sup.a        (and specific activity.sup.b)              Total    Cytoplasmic                                PeriplasmicActivity  Clone    extract  fraction fraction______________________________________CMCase.sup.c     pEC2     0.063    0.063    0.00949              (0.215)  (0.167)  (0.529)     pcEC2    0.00472  0.00222  0.00264              (0.0152) (0.006)  (0.148)B-lactamase.sup.d     pEC2     815.93   47.18    700              (2550)   (125.2)  (39002)     pcEC2    911.7    53.45    745              (2348)   (117.3)  (35975)B-galactosidase.sup.e     pEC2     0.923    1.11     0.00571              (2.88)   (2.95)   (0.32)     pcEC2    0.941    1.13     0.00663              (2.42)   (2.48)   (0.32)______________________________________ LEGEND .sup.a Proteins from total cell extracts were prepared by breaking the cells using a French press (Whittle et al., 1982). Periplasmic proteins were isolated by osmotic shock (Nossal and Heppel, 1966). Cytoplasmic proteins were prepared by rupturing the osmoticallyshocked cells with a French press. The unbracketed numbers represent the respective activity ( of enzyme/ml of cell culture) of CMCase, Blactamase and Bgalactosidase of pEC2 and pcEC2 clones. .sup.b The numbers in parentheses represent the repective specific activity (U of enzyme/mg of protein) of CMCase, Blactamase and Bgalactosidase of pEC2 and pcEC2 clones. .sup.c CMCase activity was assayed as described in MATERIALS AND METHODS, section b; U for CMCase activity is umol of glucose equivalents released per min. .sup.d Blactamase activity was determined with nitrocefin as described by O&#39;Callaghan et al. (1972); U for Blactamase activity is umol of nitrophenol acid produced per min. .sup.e Bgalactosidase activity was measured with ONPG as the substrate (Miller, 1972); U for Bgalactosidase activity is umol of o-nitrophenol produced per min. 
    
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     As will be apparent to those skilled in the art in the light of the foregoing disclosure, many alterations and modifications are possible in the practice of this invention without departing from the spirit or scope thereof. Accordingly, the scope of the invention is to be construed in accordance with the substance defined by the following claims.