Abstract:
The gene coding for a protein A-like material has been successfully cloned and expressed for the first time. The cloning of this gene with its nucleotide sequence characterization, also disclosed, enables those skilled in the art to obtain quantities of a protein A-like material nucleotide sequence for cloning in various host-vector systems. Protein A is well known as a valuable component of a variety of diagnostic test systems. The protein A-like material of the subject invention, and subfragments thereof, have the protein A properties of binding to IgG at the Fc region and activation of polyclonal antibody synthesis. Thus, these entities are useful in the same manner as protein A.

Description:
BACKGROUND OF THE INVENTION 
     Protein A is a constituent of the cell wall of the bacterium Staphylococcus aureus. One form has a reported molecular weight of 42,000 and is a major component (1.7% of total cell protein) of the cell wall. See Bjork, (1972) Eur. J. Biochem. 29:579. Measurements of frictional ratio and intrinsic viscosity of protein A in comparison to most globular proteins suggest that its shape is relatively elongated. Controlled trypsinization of the molecule reveals 4 homologous peptide domains (designated in order from the N-terminus as D, A, B, C), each of which can bind one molecule of IgG at the Fc region. See Sjodahl, J. (1977) Eur. J. Biochem. 73:343 and L Sjodahl, J. (1977) Eur. J. Biochem. 78:471. The relative binding efficiency of protein A is dependent upon a number of factors, including pH, species, class, and subclass of IgG. Because of its ability to bind to IgG without significantly affecting the affinity of immunoglobulin for antigen, protein A is widely used as an immunoabsorbent in a variety of diagnostic and basic research test systems. See U.S. Pat. No. 4,322,274. Recent interest in applications of protein A has centered around its possible clinical use in anti-cancer treatment. Sensitized peripheral blood lymphocytes, normally responsible for cytotoxicity of tumor cells, are hypothesized to be inhibited in this function by serum blocking factors which are presumed to consist of specific antigens, antibodies, antiglobulins, and immune complexes. See Barnes, B. C. (1981) Cancer Bull. 33:278. These &#34;blocking&#34; factors can be removed from sera of tumor-bearers by absorption to Staphlococcus aureus, Cowan I cells which contain protein A, and thus allow cell-mediated tumor cell toxicity to proceed in in vitro test systems. See Steele, G., Ankerst, J., and Sjogren, H. (1974) Int. J. Cancer 14:83. Protein A also activates polyclonal antibody synthesis independent of its IgG binding activity. See Sjodahl, J. and Moller, G (1979) Scand. J. Immunol. 10:593. 
     Extensive testing of protein A as an anticancer agent has been inhibited by the high cost of the material and by the presence of impurities in some protein A preparations. Should the cost of protein A preparations be significantly reduced and the purity improved, then further clinical testing of protein A for anticancer uses would proceed more rapidly. 
     BRIEF SUMMARY OF THE INVENTION 
     Disclosed herein are recombinant plasmids comprising a novel nucleotide sequence coding for the amino acid sequence of protein A-like material and the well-known plasmid vector pBR322. The sequence of this novel oligonucleotide follows. The entire sequence is contained in plasmid pAC37. Plasmid pAC37-6 contains the same entire sequence except for the last 209 nucleotide bases. The last six nucleotide bases of pAC37-6 code for the PstI recognition sequence, i.e., CTGCAG. 
     The following sequence discloses for the first time, surprisingly, an additional IgG-binding domain designated domain E near the amino terminal end of the protein A-like material. This domain is neither disclosed nor suggested by the prior art. In addition, an unexpectedly large carboxy terminal coding sequence has been discovered, which may constitute the region responsible for activation of polyclonal antibody synthesis. 
     The disclosed nucleotide sequence and fragments thereof enable persons in the art, for the first time, to obtain cloned nucleotide sequences coding for protein A-like material and fragments of protein A-like material. ##STR1## 
     Having the above data, those skilled in the art can readily appreciate the identity of other equivalent nucleotide sequences coding for molecules with substantially the same protein A-like biological activity. Thus, the scope of the subject invention includes not only the specific nucleotide sequence depicted above, but also all equivalent nucleotide sequences coding for molecules with substantially the same protein A-like biological activity. The term &#34;equivalent&#34; is being used in its ordinary patent usage here as denoting a nucleotide sequence which performs substantially as the nucleotide sequence identified herein to produce molecules with substantially the same protein A-like biological activity in essentially the same kind of hosts. Within this definition are fragments of the protein A-like material which have the property of binding to IgG at the Fc region, or fragments which have polyclonal B-cell activating activity. The protein A-like material of the subject invention, and fragments thereof, can be used in the same manner as protein A, disclosed above. 
    
    
     DETAILED DESCRIPTION OF THE INVENTION 
     Cloning of the DNA sequences coding for protein A-like material was initiated by construction of a gene bank comprising DNA sequences of the SAC genome (S. aureus, Cowan I, SAC, ATCC 12598). This was accomplished by G-C tailing using blunt-end SAC DNA fragments generated by HaelII+Alul partial restriction digestion as substrate. Digestion of 250 μg SAC DNA in 400 μl 50  mM Tris-HCl, pH 7.5: 5 mM MgCl: 1 mM dithiothreitol (DTT) with 150 units HaeIII and 200 units AluI (12 min., 37° C.) generated a broad size range of DNA fragments (2-10 kilobase pairs [kb]). From the published 42,000 molecular weight, it was estimated that the coding sequences of protein A should comprise 1.1-1.2 kb of DNA. To maximize the probability of obtaining a recombinant insert containing both the protein A coding sequences and adjacent regulatory sequences, larger fragments, 3-6 kb, were used for construction of the SAC gene bank. This DNA was extracted from a preparative agarose gel, tailed with 15°-20° C. residues with terminal transferase, and annealed to G-tailed, PstI-digested pBR322. Transformation of E. coli MS371 cells with the resulting recombinant DNA, G-tailed plasmid DNA alone, or uncut pBR322 yielded transformation efficiencies of 2.0×10 4 , 5.0×10 2 , and 2.0×10 6  transformants per 72 g plasmid DNA, respectively. Approximately 7.0×10 3  transformants were picked onto fresh tetracycline plates for screening. 
     Mini-lysate plasmid DNA preparations for 10 randomly picked transformants were digested with PstI and the sizes of the resulting DNA fragments analyzed by agarose gel electrophoresis. The results indicated that (1) 9 of 10 transformants carried recombinant DNA plasmids, (2) 7 of 9 recombinant plasmids had both PstI restriction sites regenerated by the G-C tailing procedure, and (3) the average insert length was approximately 3.0 kb. 
     The cloning vehicles of the subject invention are useful to make available for the first time and to increase the supply of the gene coding for molecules with protein A-like biological activity by replication of a transformed host. With this abundance of the desired gene, levels of protein A expression necessary to make protein A-like material available at a lower cost can be predicted. 
     Following are examples which illustrate procedures, including the best mode, for practicing the invention. These examples should not be construed as limiting. All percentages are by weight and all solvent mixture proportions are by volume unless otherwise noted. 
     EXAMPLE 1 
     MAINTENANCE AND GROWTH OF BACTERIAL STRAINS 
     Staphylococcus aureus, Cowan I (SAC, ATCC 12598) and Woods 46 (SAW, ATCC 10832) strains were obtained from the American Type Culture Collection, Rockville, Md., Both strains were grown (liquid or 1.5% agar plates) in Penassay medium (5 mg/ml Casitone, 2.5 mg/ml yeast extract, 2.5 mg/ml β-glycerophosphate, 4 mg/ml niacin, 2 mg/ml thiamine-HCl) under standard conditions. 
     E. coli MS371 was propagated in L-broth (5 g/l NaCl, 10 g/l bactotryptone, 5 g/l yeast extract). For plasmid DNA preparation, cells containing plasmids of interest were grown in M-9 media (49 mM Na 2  HPO 4 , 17 mM KH 2  PO 4 , 8.6 mM NaCl, 18.7 mM NH 4  Cl, 0.1 mM CaCl 2 , 1 mM MgSO 4 . 7 H 2  O, 0.4% glucose, 0.4% casamino acids, 2 mg/ml thiamine). 
     EXAMPLE 2 
     EXTRACTION OF DNA FROM SAC 
     Overnight cultures of SAC were diluted 1:100 with Penassay broth and allowed to grow to OD 600  =0.6. The cells were pelleted by centrifugation (5K rpm, 10 min., 2° C. with a Beckman JA10 rotor), resuspended in 20 volumes DNA extraction buffer (0.1 M NaCl; 50 mM EDTA; 10 mM Tris-HCl, pH 8.0), and frozen in a dry ice-acetone bath. 
     The frozen cell suspension was allowed to thaw at 37° C., 50 mg/ml lysostaphin (Sigma Chemical Co., St. Louis, Mo.) was added, and the suspension incubated at 37° C., 15 min. Protease K (40 mg/ml) and SDS (0.5%) were added and the mixture incubated at 37° C., 1 hour. The lysate was then extracted with phenol:chloroform (1:1) saturated with DNA extraction buffer. The SAC DNA solution was adjusted to 0.95 g/ml CsCl and banded by centrifugation (44 K rpm, 48 hours, 23° C. with a Beckman Ti60 rotor). The DNA was then harvested with a syringe and 21 g needle by side puncture. The DNA was dialyzed against TE buffer (10 mM Tris-HCl; 1 mM EDTA, pH 8.0), phenol:chloroform-extracted as before, and precipitated twice with 2 volumes ethanol. Yields of SAC DNA ranged between 700-800 mg DNA per gram wet weight of cells. 
     EXAMPLE 3 
     RESTRICTION ENZYME DIGESTION 
     All restriction endonucleases were purchased from Bethesda Research Laboratories, Bethesda, Md. or New England Biolabs, Beverly, Mass. Unless otherwise indicated, restriction digests, described herein, were carried out at DNA concentrations of 100-400 μg/ml, 2-4 units enzyme per μg DNA, 2-3 hours, 37° C., in buffer systems recommended for each enzyme by the respective company. 
     EXAMPLE 4 
     ELECTROPHORESIS AND EXTRACTION OF DNA FRAGMENTS 
     Agarose gel electrophoresis was carried out using a 2×Tris-acetate gel buffer (80 mM Tris-HCl, pH 8.0., 40 mM NaC 2  H 3  O 2  ; 36 mM NaCl; 2 mM Na 2  EDTA) in the gel and 1× buffer for the run. Analytical gels were routinely run as &#34;submarine gels&#34; in a horizontal gel box. Preparative gels were routinely run in an EC Model 470 gel box. DNA bands were visualized by ethidium bromide (EtBr) post-staining (0.5 mg/ml in 1×gel buffer) and use of a U.V. transilluminator Model TM-36 from Ultra-Violet Products, Inc., San Gabriel, Ca. 
     Extraction of DNA from preparative agarose gels was initiated by visualization of the positions of EtBr-stained bands of a single gel lane. Gel slices containing DNA fragments of interest were diced manually and passed through a 20 g needle with 11/2-2 volumes DNA gel extraction buffer (0.5 M NH 4  C 2  H 3  O 2 , 10 mM EDTA, 10 mM Mg(C 2  H 3  O 2 ) 2 , 0.1% SDS). An equal volume of phenol saturated with 1 mM NH 4  C 2  H 3  O 2 , 10 mM EDTA was added and extraction carried out in Eppendorf tubes) (trademark of Brinkman Instruments) on a rotary shaker at 23° C. overnight. The tubes were then placed on ice for 30 min. prior to separation of the aqueous phase by microcentrifugation. Extraction of the aqueous phase with the saturated phenol solution was repeated 3-4 times, followed by chloroform extraction and ethanol precipitation. Routine recovery of DNA fragments smaller than 15 kb was about 40%. 
     EXAMPLE 5 
     TAILING AND ANNEALING OF PLASMID AND Insert DNA 
     Construction of recombinant plasmids was facilitated by G-C tailing (Stein, I., Catterall, J., Woo, S., Means, A., O&#39;Malley, B. [1978]Biochemistry. 17:5763). PstI-digested and agarose gel-purified pBR322 DNA was tailed with approximately 14 G residues in a 100 μl reaction under the following conditions: 100 μg/ml DNA, 20 μM dGTP, 200 mM K/cacodylate, 1 mM CoCl 2 , 1 mM β-mercaptoethanol (B-SH), 15 units terminal deoxynucleotidyl transferase (P. L. Biochemicals, Inc., Milwaukee, Wis.) 37° C., 30 min. The reaction was terminated by the addition of 2 μl 100 mM EDTA, 2 μl 5 M NaCl, 2 μl 20% SDS and phenol:chloroform (1:1) extraction. The resulting G-tailed plasmid DNA was passed over a G-50 Sephadex column and precipitated with ethanol. 
     Target SAC DNA fragments of average 3-5 kb length were tailed with 15°-20° C. residues in a 30 μl reaction under the following conditions: 4-5 μg SAC DNA, 20 μM dCTP, 200 mM K/cacodylate, 1 mM CoCl 2 , 1 mM β-SH, 4.5 units terminal deoxynucleotidyl transferase: 37° C., 12 min. Termination of the reaction and treatment of C-tailed SAC DNA was carried out as described above. Annealing of plasmid and target SAC DNA was initiated by mixing 2.5 μg plasmid and 4.0 μg target SAC DNA in 300 μl 10 mM Tris-HCl,pH 8.0; 1 mM EDTA., 100 mM NaCl; and heating for 10 min. at 68° C. The annealing solution was then allowed to incubate 1 hour at 55° C., 1 hour at 23° C., and was stored at 4° C. until needed. 
     EXAMPLE 6 
     LIGATION OF DNA FRAGMENTS 
     Ligation of staggered-end DNA fragments was carried out with 100-200 units/ml T 4  DNA ligase (Bethesda Research Laboratories); 66 μM ATP; 66 mM Tris-HCl, pH 7.6; 6.6 mM MgCl 2  ; 10 mM dithiothreitol; at 12° C., 12-16 hours. 
     EXAMPLE 7 
     Transformation OF E. COLI MS371 Cells 
     Fresh overnight cultures were diluted 1:100 in L-broth and allowed to grow at 37° C. with shaking to OD 600=0 .1-0.15. The cells were pelleted (5 min. 5K rpm, 5° C. in a JA20 rotor in a Beckman J2-20 centrifuge), resuspended in half the original volume of ice-cold 50 mM MnCl 2  ; 10 mM NaC pH 5.6; and allowed to stand at 0° C., 20 min. Following pelleting of the cells as above, they were resuspended in ice-cold 100 mM MnCl 2  ; 75 mM CaCl 2  ; 10 mM NaC 2  H 3  O 2 , pH 5.6. A 0.1 ml aliquot of cells was mixed with 10 μl DNA transformation solution and allowed to sit on ice 40 min. The cells were then subjected to heat shock (2.5 min., 25°-30° C.) and 1.5 μl 2.0 M Tris-HCl, pH 7.4, and 0.5 ml L-broth per 0.1 ml cell aliquot were added. The cells were then plated in 15-25 μl aliquots on 1.5% agar L-broth plates supplemented with 10 μg/ml tetracycline (Sigma) and incubated overnight at 37° C. Transformation efficiencies of 1.0×10 7  colonies per μg pBR322 DNA were routinely observed. 
     EXAMPLE 8 
     MINI-LYSATE PLASMID DNA PREPARATIONS 
     Mini-lysate plasmid preparation was initiated by addition of 1 ml of fresh overnight culture to 9 ml L-broth, supplemented with 1% glucose and allowed to grow with shaking at 37° C. to an OD 550  of 1.0. Chloramphenicol was then added to 150 μg/ml and the culture incubated for 12-16 hours at 37° C. The cells were then pelleted by centrifugation (5 min., 3K rpm, 23° C. in an RC-3 centrifuge), resuspended in ice-cold TE buffer, and transferred to a 1.5 ml eppendorf tube to be repelleted by centrifugation. The resulting cell pellet was resuspended in 50 mM Tris-HCl.pH 8.0; 50 mM EDTA; 15% sucrose (wt/vol) by vortexing. To the cell suspension, 10 μl of 10% SDS were added and incubated at 70° C., 10 min. To the resulting lysate, 62.5 μl ice-cold 4 M potassium acetate was added and the lysate allowed to stand for at least 2 hours on ice. Following centrifugation the supernatant volume was adjusted to 0.5 ml with H 2  O and the DNA precipitated with 2 volumes absolute ethanol. The DNA was then resuspended in 100 μl TE, the salt adjusted to 0.1 M with NaCl, and re-precipitated with two volumes ethanol prior to restriction enzyme analysis. 
     EXAMPLE 9 
     LARGE-SCALE PLASMID DNA PREPARATIONS 
     Overnight 25 ml cultures were grown in L-broth supplemented with 10 μg/ml tetracycline. To one liter M-9 media, 5 ml of the overnight culture were added and allowed to grow at 37° C. in a rotary incubator (200 rpm) until an OD 600  value of 0.6 was reached. 250 mg/liter chloramphenicol (Sigma) was then added and the culture allowed to shake for 12-16 hours at 37° C. The cells were then harvested by centrifugation (6000 rpm, 20 min., 2° C. in Beckman JA-10 rotor), and the pellets washed once with ice-cold TE buffer. The washed pellets were then either frozen at -60° C. or immediately extracted. Preparation of cleared lysates was initiated by suspending the cell pellet in 6.25 ml per liter original culture of 25% sucrose in 50 mM Tris-HCl, pH 8.0, and then adding 1.5 ml of a freshly made 10 mg/ml lysozyme (Sigma) solution. After continuous swirling of the suspension on ice for 5 min., 1 25 ml of 0.5 M Na 2  EDTA, pH 8.0, was added and swirling of the suspension on ice continued for 5 min. Ten ml of a 10×Triton (10 ml 10% Triton X-100; 125 ml 0.5 M EDTA, pH 8.0; 50 ml 1.0 M Tris-HCl; pH 8.0: and 800 ml H 2  O) per liter original culture volume was added and the suspension swirled on ice for 15 min. The lysate was then subjected to centrifugation (19 K rpm, 4° C., 30 min. in a JA-20 rotor) and the supernatant transferred to a volumetric cylinder. 0.95 g/ml CsCl was dissolved in the supernatant and 1/10 the volume of 10 mg/ml EtBr in TE buffer was added. Separation of plasmid and chromosomal DNA was accomplished by centrifugation with a Beckman Ti 50.2 rotor (23° C., 44K rpm for 24 hours followed by 36 hours at 38 K rpm). 
     The plasmid DNA band on the gradient is visualized with a U.V. lamp and harvested with a syringe by side puncture using a 21 g needle. Removal of EtBr is carried out by repeated isobutyl alcohol extraction. The plasmid solution is then dialyzed overnight against TE buffer, the salt concentration adjusted to 0.1 M NaCl and precipitation of DNA carried out with 2 volumes of absolute ethanol. 
     EXAMPLE 10 
       125  I-IGG-PROTEIN A BINDING ASSAY 
     Expression of protein A-like activity in bacterial colonies was detected by binding of 125I-IgG to colony lysates immobilized on nitrocellulose filters. Recombinant plasmid-bearing E. coli, SAC (positive control) and SAW (negative control) cells were picked and streaked onto nutrient agar plates and allowed to grow overnight. Nitrocellulose filter discs (BA85, 87 mm, Schleicher and Schuell, Keene, N. H.) were carefully laid on the plates to absorb the underlying colonies, and the filters lifted and allowed to dry by blotting on Whatman 3 MM paper. Lysis of filter-bound cells was accomplished by laying the filters (colony side up) on sheets of Whatman 3MM filter paper saturated with 0.5 M NaOH and allowing lysis to proceed for 10 min. at 23° C. Following lysis, the filters were blot dried and neutralized on filter paper saturated with 1.0 M Tris-HCl, pH 7.0. The filters were again blot dried and pre-treated with protein binding solution (10 mM Tris-HCl, pH 7.0; 100 mM NaCl; 5 mM EDTA; 0.13% NP40; 0.1% SDS: 0.1% sodium deoxycholate: 0.2% Ficoll 400; 0.3% gelatin) for 4-6 hours at 23° C. on a rotary platform shaker. After pre-treatment, the filters were transferred to a 1-liter beaker containing a 4.5 ml/filter protein-binding solution. Binding of  125  I-IgG (Goat Anti-rabbit, New England Nuclear, Boston, Mass.) was carried out by the addition of 5×10 6  cpm/ml  125  I-IgG to the beaker and allowing binding to occur at 4° C. overnight with constant rotary shaking. Washing of the filters was accomplished by repeated washing with 500 ml protein-binding solutions: the first wash carried out at 4° C., and 2-3 additional washes carried out at 23° C. The washed filters were then dried by blotting and detection of  125  I-IgG binding accomplished by radioautography, using Kodak XAR-5 film and two DuPont Cronex Lightning-Plus enhancement screens. 
     EXAMPLE 11 
     DNA SEQUENCING 
     DNA sequence determination was carried out with minor modification of procedures described by Maxam and Gilbert (Maxam, A. and Gilbert, W. [1977]Proc. Nat&#39;l. Acad. Sci. USA, 74:560) and Heidecker et al. (Heidecker, G., Messing, J., and Gronenborn, B. [1980]Gene 10:69). 
     EXAMPLE 12 
     SCREENING FOR EXPRESSION OF PROTEIN A-LIKE Material in E. coli Transformants 
     To test for the expression of sequences coding for protein A-like material within the recombinant SAC gene bank, the colonies from 50 plates of 52 colonies each (2,600) were lifted on nitrocellulose discs and assayed for  125  I-IgG binding. Filters containing SAC and SAW colonies were included in the assay as positive and negative controls, respectively. To assess the sensitivity of the assay, serial dilutions of purified protein A (Pharmacia, Piscataway, N.J.) were spotted onto a nitrocellulose disc and assayed in parallel with the test filters. The routine sensitivity for the assay was found to vary over a range of 1.0 to 0.01 ng with purified protein A. Filters containing SAC and SAW cells yielded positive and negative autoradiographic signals, respectively. A single transformant colony bound significant  125  I-IgG in this and subsequent assays. This colony was picked for further analysis. The plasmid contained in this colony was designated pAc37. 
     EXAMPLE 13 
     DETERMINATION OF THE PROTEIN A-LIKE GENE Domain Within the pAc37 Insert 
     Restriction endonuclease analysis of pAc37 plasmid DNA indicated the presence of PstI insert fragments of 3.1, 2.3, 1.9, and 0.65 kb length. pAc37 plasmid DNA was digested with PstI, re-ligated with T4 ligase, and used to transform E. coli MS371 cells. The resulting transformants were screened by the  125  I-IgG-binding assay as described in example 12. 
     Of 322 transformants, 10 positive  125  I-IgG-binding colonies were obtained and were found to have recombinant plasmids containing a 1.9 kb PstI insert. When recombinant plasmid DNAs from 12 randomly picked non- 125  I-IgG-binding transformant colonies were analyzed they were found to contain one or more PstI fragments from pAc37, but not a 1.9 kb fragment. It was concluded that at least a portion of the protein A-like coding sequences reside within a 1.9 kb PstI fragment of pAc37. One positive colony containing a recombinant plasmid with a single 1.9 kb insert, designated pAc37-6, was picked for further analysis. 
     EXAMPLE 14 
     IDENTIFICATION OF THE PROTEIN A-LIKE CODING Sequences Within pAc37-6 DNA 
     Final determination of the presence of protein A-like coding sequences within the PstI 1.9 kb fragment of pAc37-6 DNA was accomplished by DNA sequence determination. The pAc37-6 DNA was digested with HindIII, labeled with γ 32  P-ATP and polynucleotide kinase, and subsequently digested with PstI. Sequence determination of a portion of the 0.6 kb HindIII/PstI fragment indicated sequence colinearity with the known amino acid sequence of the B-C junction of the protein A molecule. The position of the sequences coding for the B-C junction of the protein A-like material within the insert made it likely that the 1.9 kb insert of pAc37-6 plasmid DNA contained most of the sequences coding for the protein A gene, including the ribosome binding site, and 5&#39; regulatory sequences. 
     EXAMPLE 15 
     PURIFICATION OF PROTEIN A-LIKE MATERIAL FROM E. coli MS371 (pAc37-6), NRRL B-15131 
     E. coli MS371 (pAc37-6) is lysed with 0.1 N NaOH and centrifuged. The supernatant is removed and 25 mM monobasic sodium phosphate is added and the solution adjusted to pH 7.0 with 1 M HCl. The protein solution is dialyzed against 25 mM sodium phosphate pH 7.0, then clarified by centrifugation. 
     The solution is applied to an IgG-Sepharose column (30 ml bed volume per 1.3 gm of protein) and the column washed with 0.1 M sodium phosphate pH 7.0 until no protein, as determined by A 280 , elutes from the column. 
     Protein A-like material is eluted with 0.1 M glycine.HCl. The purified protein is concentrated by precipitation with 80% saturated (NH 4 ) 2  SO 4 , dialyzed versus 10 mM sodium phosphate pH 7.0, and stored frozen. 
     The purification of protein A-like material from E. coli MS371 (pAc37), NRRL B-15127 can be accomplished by using the procedure described above. 
     EXAMPLE 16 
     ISOLATION OF NUCLEOTIDE SEQUENCES CODING for fragments of the Amino Acid Sequence Coding for Protein A-Like Material from E. coli MS371 (pAc37-6), NRRL B-15131 
     Restriction enzymes can be used to cleave the nucleotide sequence coding for protein A-like material in order to isolate essentially pure fragments of the coding region that are capable of coding for amino acid sequences with biological activities similar to those of protein A. For example, cleavage of pAc37-6 DNA with RsaI restriction endonuclease will yield an oligonucleotide that is 1,199 nucleotides long and that codes for a polypeptide containing domains E, D, A, B, and C. Digestion with other restriction enzymes such as HinfI, or a combination of enzymes such as HindIII and Sau3A, can be used to generate essentially pure, well-defined oligonucleotide fragments that code for amino acid sequences with biological activities similar to those of protein A. 
     The desired oligonucleotide fragments are isolated in their essentially pure form by preparative agarose gel electrophoresis as follows: Agarose is dissolved to 1% in 2x E buffer (0.08 M Tris.HCl, pH 7.8; 0.01 M NaC 2  H 3  O 2  ; 0.002 M EDTA) and poured into a Bio-Rad (Richmond, Ca.) slab gel apparatus. Samples are dissolved in 10 mM Tris.HCl, pH 8.0; 0.1 mM EDTA and the samples are run at constant power with 2×E running buffer. 
     After electrophoresis, one lane is cut from the gel, stained with ethidium bromide (0.5 μgm/ml) and the DNA bands visualized under ultraviolet light. The band of interest is cut from the rest of the gel and macerated before passing it through a 20 guage needle. An equal weight of extraction buffer (10 mM Tris.HCl, pH 8.0; 2 mM EDTA: 1 M NaCl) is then added and mixed with the gel. The mixture is incubated at 47° C. for 16 hours and the agarose pelleted at 100,000×g for 1 hour. The supernatant is then made 30 μgm/ml in tRNA and extracted with phenol until no agarose is visible at the interface. The DNA is then ether extracted and ethanol precipitated. Gel buffers and extraction procedures can be varied by one skilled in the art to recover the desired DNA fragments. 
     EXAMPLE 17 
     SYNTHESIS OF NUCLEOTIDE SEQUENCES CODING for the Amino Acid Sequences of Domains E, D, A, B, and C of Protein A-Like Material 
     Once the nucleotide sequence coding for a particular amino acid sequence has been determined, i.e., by cloning and sequencing as shown in previous examples, then the oligonucleotide coding for the amino acid sequence can be synthesized chemically. (See, for example, Edge, M. D., et al. [1981]Nature 292:756-762.) Thus, fragments of the coding region, or the entire coding region for a protein A-like molecule, can be synthesized and isolated in their essentially pure forms; this includes those regions of the coding sequence coding for domains E, D, A, B, and C. 
     Domains E, D, A, B, and C, each alone, or in various combinations, are useful in the same manner as protein A to bind IgG in diagnostic test systems, as described previously. 
     EXAMPLE 18 
     Cloning and Expression of the Nucleotide Sequences Coding for the Amino Acid Sequences of Domains E, D, A, B, and C of Protein A-Like Material 
     The essentially pure nucleotide sequences coding for protein A-like material or for biologically active fragments of protein A-like material, isolated and synthesized as described in examples 16 and 17, respectively, can be ligated into appropriate restriction enzyme sites in an expression cloning vector. If necessary, sites can be added to nucleotide sequences using linker molecules. (See, for example, Norris, K. E., et al. [1979]Gene 7:355-362.) The ligated DNA can then be used to transform a host organism. Previous work by others has shown that expression of the cloned nucleotide sequence would be expected. (See, for example, Doel, M. T. et al. [1980]Nuc. Acids Res. 8: 4575-4592: Roberts T., et al. [1979]Proc. Nat. Acad. Sci. 76:760-764; Guarente, L., et al. [1980]Cell 20: 543-553.) The biologically active material that is expressed can then be purified as described in example 15. 
     Plasmids pAc37 and pAc37-6 have been deposited in an E. coli host in the permanent collection of the Northern Regional Research Laboratory (NRRL), U.S. Department of Agriculture, Peoria, Ill., U.S.A. Their accession numbers in this repository are as follows: 
     E. coli MS371 (pAc37)--NRRL B-15127: Deposited on Aug. 18, 1982 
     E. coli MS371 (pAc37-6)--NRRL B-15131: Deposited on Aug. 18, 1982 
     E. coli MS371--NRRL B-15129: Deposited on Aug. 18, 1982 
     Plasmid pBR322 is a well-known and available plasmid. It is maintained in the E. coli host ATCC 37017. Purified pBR322 DNA can be obtained as described in Bolivar, F., Rodriquez, R. L., Greene, P. J., Betlach, M. C., Heyneker, H. L., Boyer, H. W., Crosa, J. H., and Falkow, S. (1977) Gene 2:95-113; and Sutcliffe, J. G. (1978) Nucleic Acids Res. 5:2721-2728. 
     NRRL B-15127, NRRL B-15131, and NRRL B-15129, are available to the public upon the grant of a patent which discloses these accession numbers in conjunction with the invention described herein. It should be understood that the availability of these deposits does not constitute a license to practice the subject invention in derogation of patent rights granted for the subject invention by governmental action. 
     There are other well-known hosts which can be used instead of E. coli MS371, for example, B. subtilis, Streptomyces species, and yeast. 
     Also, it is within the skill of those in the art to vary the conditions required to grow cells, extract DNA, perform restriction enzyme digestions, electrophorese DNA fragments, tail and anneal plasmid and insert DNA, ligate DNA, transform E. coli cells, prepare plasmid DNA, perform an IgG-binding assay, prepare protein lysates, electrophorese proteins, and sequence DNA.