CA2215528C - Method for diagnosing a patient for chlamydia - Google Patents

Method for diagnosing a patient for chlamydia Download PDF

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CA2215528C
CA2215528C CA002215528A CA2215528A CA2215528C CA 2215528 C CA2215528 C CA 2215528C CA 002215528 A CA002215528 A CA 002215528A CA 2215528 A CA2215528 A CA 2215528A CA 2215528 C CA2215528 C CA 2215528C
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glxa
monoclonal
igg
antibody
chlamydial
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Alex B. Macdonald
Elizabeth Sutton Stuart
Ling-Ling An
Myron Whipkey
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University of Massachusetts UMass
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Abstract

A method of detecting chlamydia in an extracellular sample is provided which comprises contacting the sample with an idiotypic antibody to GLXA to form an immunocomplex and detecting the immunocomple x.

Description

METHOD FOR DIAGNOSING A PATIENT FOR CHLAMYDIA

BACKGROUND OF THE INVENTION
This invention relates to a method for diagnosing a patient for the presence of Chlamydia.
Chlamydial infection is a diverse group of conjunctiva), genital, respiratory, and neonatal infections occurring primarily on mucosal surfaces. The etiologic agent of the infection is an obligate intracellular bacterial parasite of eukaryotic cells, chlamydiae. There are four genetically different species in this genus, with certain similarities in morphology, intracellular developmental cycle and antigenic re-sponses: Chlamvdia trachomatis. Chlamydia t~sittaci. Chlamydia pneumoniae. and Chiamydia Percorum. The infection by C.trachomatis is limited to humans.
Fifteen serovars are differentiated based on the antigenic variations of the major outer membrane protein (MOMP) (Grayston and Wang,J. Infect. Dis:, 132:87, 1975).
Serotypes D-K, are the most common cause of sexually transmitted venereal diseases. Conservatively, more than 4 million cases of chlamydial sexual infections occur each year in the United States making it more prevalent than all other sexually transmitted diseases combined. The diseases include nongonococcal urethritis, mucopurulent cervicitis, acute epididymitis, ectopic pregnancy and pelvic inflammatory disease (PID, endometritis, salpingitis, parametritis and/or peritonitis).
The infection in women can be quite damaging: Among 250,000 cases of pelvic inflammation diseases caused by this organism in the U. S. each year, 10% lead to infertility. When infants are bom to chlamydia-infected mothers, they are at high risk of developing inclusion conjunctivitis and pneumonia. C. trachomatis serovars A, B, Ba, and C cause trachoma, an infection of conjunctiva) epithelial cells. The chronic and secondary infections induce the infiltration of subepithelial lymphocytes, forming follicles and the invasion of fibroblasts and blood vessels to the cornea, leading to blindness. On the other hand, the formation of the scar and malformation of the eyelid, causing trichiasis' constant scraping of the cornea by the eyelash can also WO 96/29604 PCT/US961026I'7 lead to corneal opacification and blindness: There are approximately 500 million trachoma cases in the world, and between 7 and 9 million are now blind because of its complications making it the world's leading cause of preventable blindness. The prevalence of active trachoma is high in early age. There are 80 million children in need of treatment. It has been an enormously important health problem in the Middle East, North Africa, South Asia and North India.
C. psittaci mainly affects animals and birds. It had, and still has a great economic impact in dairy, wool and meat industries.' There are 9 serovars from mammalian species, 7 serovars from avian species and 2 biovars from koala bears. Mammalian serovar 1, 2, 3, and 9 infect cattle and sheep, causing a wide range of disorders from placenta and fetus infection and other reproductive problems, including polyarthritis-polysistitis, encephalomyelitis, conjunctivitis as well as intestinal infections. Although numerous attempts have been made to produce vaccines, only modest success has been achieved (Schnorr, J. Am. Vet.
Med. Assoc. 195:1548, 1989). Serovars 4, 5, and 6 are the causes of abortions, pneumonia and polyarthritis in porcine species. Serovar 7 represents chlamydial strains of feline conjunctivitis, rhinitis and pneumonitis and serovar 8 includes guinea pig inclusion conjunctivitis. The avian strains often cause human infection in bird handlers and poultry processing workers.
C. pneumoniae is a newly identified species. To date, one serovar has been identified, TWAR (Grayston, Proceedings of the Seventh International Symposium on Human Chlamydial Infections, Pg. 89, 1990). Current evidence suggests that C. pneumoniae is a primary human pathogen that is transmitted from human to human and causes about 10-20% of community acquired pneu-monia in adults. It has become the main causative agent of human respiratory diseases such as pneumonia, bronchitis, pharyngitis, and sinusitis and a possible agent in reactive arthritis. Epidemics have occurred in hospitals, in the military and families. The serological finding from many countries have shown that 50-55% of adults with antibody against TWAR antigen are specific for C. pnueun-oniae. It is the major bacterial cause of illness in newborn. The infection to elderly persons and those with chronic diseases may cause serious illness or even death.
Chlamydia pecorum was identified as a new species in 1992. It is °
prevalent in cattle, sheep and swine and a number of exotic birds and invertebrates. In cattle it causes encephalomyelitis, upper respiratory disease and pneumonia. Whereas in sheep, it has been isolated in Iambs with polyarthristis. It is widespread and pathogenicity in animals has still not been .
determined for some species (Storz et al, Proceedings of the Eight International Symposium on Human Chlamydia Infections, Pg 563, 1994).
The pathogenicity of chlamydial infection is not well understood. It is long known that different individuals infected by these serovars exhibit different clinical manifestations. It has been proposed that it was likely due to the variation of the host immune response. It has been shown that immunologic response to the synthetic Th/B cell epitopes in the various inbred strains of mice is different, indicating that the T helper epitope is recognized in the context of the multiple major histocompatibility complex.
The target of chlamydial invasion are typically epithelial cells of a host. It is still not certain' how the chlamydial elementary bodies (EB), (a sporelike, spheri-cal particle, about 300 nm in diameter), enter the host cell: receptor-mediated endocytosis, and/or non-specific high affinity absorption. It has been reported that two proteins, 18 and 32 kD of C. trachomatis bind to Hela 299 cell mem-brane preparations. Recently, another heat-liable protein membrane protein, 38kD, was proposed as binding to Hela cell line, suggesting a ligand like mechanism. It has also been proposed that since chlamydia have the ability to infect a wide variety of mammalian cells in vitro, there must be some adherence mechanism for the establishment of the infection. The major outer membrane protein was proposed as such an adhesin. Recently, it has been demonstrated that a heparin sulfate-like glycosaminoglycans present on the surface of chlamydia organisms is required for attachment to host cells. The receptors on the host cells have also been studied. It was suggested that proteins, 18,000 and 31,000 kD from Hela cells are the receptors due to trypsin sensitivity for the EB
specfic binding. It also has been shown that C. trachomatis and C. pneumoniae bind specifically to a lipid on Hela cells. Nuclear magnetic resonance spectros-copy analysis and atom bombardment mass spectrometry show that it was phosphatidylethanolamine (PE). At the same time ganglia-series glycolipids were found specifically bound to EBs. All those findings suggest that the mechanism of endocytosis by epithelial host cells is still a matter of uncertainty. Once the EBs enter the host cells by endocytosis, depending upon conditions, they are trans-formed into a metabolically active, non-infectious reticulate body (RB). The prime purpose of RBs is intracellular replication by binary fission using host metabolites. This occurs in a membrane-bounded vesicle, termed an inclusion.
This inclusion (endosome) can resist the fusion with the lysosomes of host cells.
Each RB eventually gives rise to one or more EBs which can initiate another infectious cycle. Host cells may be lysed by release of inclusion bodies or undamaged by exclusion body excytosis. Surface antigens are thought to direct both phagocytosis and evasion of phagolysosomal fusion.
Surface components of chlamydia actively interact with host cells and with the host's immune system. They are believed to account for the attachment, endocytosis and the immune response, but the exact nature and regulation of these interactions has not yet been fully identified. Several distinct antigenic components of C. trachomatis, C. psittaci and C. pneumonia have been in-vestigated including the identification, characterization and function in chlamydial infection. Moreover, it is of importance to determine the mechanism of infection and determine the protective antigens. Surface exposed antigens are the main targets of much research since they are accessible to the immune or other defense systems. The antigens most actively investigated include major outer membrane proteins (MOMP) chlamydial lipopolysaccharide, 60-kD heat shock protein (~ iSPO 60) adhesins and a glycolipid exoantigen termed the exoantigen (GLXA).
in the outer membrane of chlamydia there are three cysteine-rich proteins 57, 40, a:~d 12.5 kD which resembles the matrix proteins of gram-negative bacteria. The 57 and 12.5 kD proteins can not be found in the replicating form of the bacteria RBs. As the major outer membrane protein (MOMP), 40 kD, is ' abundant in both infectious EBs and RBs. In RBs, the protein could function as pore-forming proteins that permit exchange of nutrients for the reticulate bodies.
Genetic and molecular characterization have shown that this protein is composed of four variable segments (VS) interspersed among five constant segments.
Those variable segments are surface exposed and have the determinants of serovar, subspecies and species specificity.
The studies on immune responses to this protein are mostly carried out by immunization of animals with purified protein. In vitro neutralization experiments have been conducted using the mixture of poly or monoclonal antibodies specific to MOMP and EBs to infect cell culture. These experiments indicate that the antibodies specific to MOMP protein or one single epitope prevent the inclusion bodies formation in cell culture. The mechanism of the neutralization does not involve inhibition of the attachment or penetration, but rather interFere with the process after internalization. Using monoclonal antibodies generated by the whole elementary bodies of serovar B, the monoclonal antibodies which recog-nized the immune accessible MOMP epitope in dot blot assays, neutralized the infectivity of organisms of monkey eyes. The protection was serovar-specific.
In a later experiment by using Fab fragments of the monoclonal antibody, it has been further demonstrated that monovalent Fab neutralized the infection by preventing the attachment to Syrian hamster kidney (HaK) cells. Confirming that the protection is not due to the aggregation of bivalent IgGs. T cell epitopes of MOMP have also been investigated. T cell proliferation responses were found in spienic T cells obtained from A/J mice immunized with MOMP in the presence of 6 ' R'O 96/29604 PCTlU596/02617 overlapping synthetic peptides which represent primary sequence of serovar A
MOMP. The synthetic peptides which produced T cell response correspond to surface-accessible serovar-specific epitopes located in variable domains (VD) VD
' i and VD IV. By using a similar approach, it was found in BALB/cByJ mice that VDIII fragment is T cell dependent. It also has been shown that by using chimeric T/B cell peptides derived from two epitopes of MOMP, one is a conserved T
helper cell epitope and the other is a serovar A specific neutralizing epitope.
Some mice immunized with this peptide produced high titered serum-neutralizing antibodies, while others did not. Although MOMP has been a most intensively studied surface antigen and the neutralization antisera has been produced in experimental animals, there are still many unsolved questions regarding thr:
immune response. For example, the neutralization of infection is serovar specific, thus, it is limited as a vaccine candidate. The neutralization is still limited to in yitro studies, and there has been no convincing in vivo protection from challenge by immunization with any MOMP or chimeric epitopes known.
It has long been known that a chlamydia genus specific antigen was a glycolipid (Dhir et al, J. Immunoi. 109: 116-122, 1972). Much later, it was found that iipopolysaccharide (LPS) was in the outer membrane of both EBs and RBs of chlamydia. It has a chemical structure similar to enterobacterial LPS of the Re chemotype (Nurminen et al, Science, 220: 1279-1281, 1983). The monoclonal antibodies prepared by immunization with EBs of serovar L2 were specifically against LPS of chlamydia, but not LPS from N Gonorrhoea. S. typhimurium, or E. coli. However, antibodies produced by S. typhimurium Re LPS or lipid A
recognized chlamydial LPS (Caldwell and Hitchcock, Infect. Immun., 44: 306, 1984). This demonstrated that chlamydial LPS has an unique antigenic domain compared to other gram-negative bacteria. Further characterization has shown that a chlamydia-specific domain contained in its saccharide portion, 3-deoxy-D-_ manno-2-octulosonic acid (KDO) with a sequence of akDO (2-8)- akDO(2-4) cr-kD0(kD03). The 2.8 linked moiety is the structural characteristic of chlamydial LPS. Studies have also been carried out in the distribution and the relocation of LPS on the outer membrane during the developmental cycle. By immunostaining with a monoclonal antibody it was shown that LPS is loosely bound in the membrane du: ing the developmental cycle, and not shed into media.
Chlamydial LPS was thought to be an ideal antigen for the vaccine candidate because of its abundance on the surface and its being antigenic. LPS
was suspected as an important virulent determinant in the early steps of the infection and the antibodies specific to it serve some function in resolving the chlamydial infection. However, little is known concerning the biological function of LPS or the immunological response to it. It appears that the antibodies which are specific to LPS only have been useful in the diagnosis of chlamydial infection and location of LPS, but not effective in resolving an infection.
Other genus-specific chlamydial antigens are 57 to 60 and 75 kD proteins which have been identified as related to the heat shock protein (HSP) family.
This was done by comparing the sequence of the operons encoding these proteins to the groE stress response operon of E. coli or B. meQaterium. The antigenic identity of 57 kD protein was confirmed by the reaction with anti-HSP-60 antiserum. The 60 kD protein elicited an ocular hypersensitivity response in immune guinea pigs, which was characterized by a predominantly mononuclear macrophage and lymphocyte cellular infiltration (Watkins, et al, Proc. Natl.
Acad.
Sci. USA 83: 7580, 1986, Morrison et al, S. Exp. Med. 169: 663, 1989). This was the first indication that an antigen is responsible for delayed hypersensitivity in chlamydial ocular infection. The precise involvement of this protein in stimulat-ing immunopathogenic responses in human chlamydial diseases has not been determined. There is evidence that shows a certain percentage of sera taken from women with PID, ectopic pregnancy and tubal infertility have high anti-chlamydial antibodies reacting to chlamydial HSPO-60 heat-shock protein.
However, not every patient serum which has high titer to chlamydia reacts with it, indicating that either HSP-60 is not surface exposed or antigenicity is MHC

restricted.
The 75-kD protein was found preferentially transcribed during heat stress of chlamydial organisms. The monospecific antibodies from rabbits raised against 75-kD protein were found to bind to the organism and neutralized the infection in vitro. It is an exposed antigen in the outer membrane.
" Genus-specific glycolipid exoantigen (GLXA) was originally isolated from the supernatants of chlamydia infected cell cultures (Stuart and MacDonald, Current Microbiology, 11: 123, 1982). it has been characterized chemically, biologically and serologically in recent years (Stuart and MacDonald, Proceed-ings of the Sixth International Symposium on Human Chlamydia Infections, p167, 1986, Stuart et al, Immunology, 67: 527, 1987). Mass spectrographic analysis indicated that GLXA contains polysaccharides: gulose, (not glucose), mannose and possibly gaiactose, while the lipid component has fatty acids of chain length C17 and C18:1. There is no KDO or lipid A found in its structure. It is produced and released from the infected cells during the growth cycle in vitro.
Transmis-sion electron microscopy utilizing colloidal gofd-conjugated goat anti-mouse second antibody to detect the specifically bound monoclonal antibody revealed that GLXA is mostly extracellular 48 hours after the infection (Stuart et al, immunology, 74: 747, 1991 ) which is different from that found for chlamydial LPS. Human sera from patients with clinically defined lymphogranuloma venereum (LG~ contain IgG antibodies which recognize GLXA (Stuart and MacDonald, Immunology, 68: 469, 1989), demonstrating the immunoaccessibifity in the natural infection. But, there was little information on its function in the chlamydial infection and the immune response to it. The overall immunological reaction to chlamydial antigens is not well understood. It is still not known how the chlamydia evade the~host immune surveillance. Antibodies found speck to chiamydial antigens in infected human patients have shown little protection for later infection. Although chlamydia mainly affects mucosal surfaces, the clinical relevance of the IgA immunity to it has not been completely described. The WO 96!29604 PCT/US96/02617 feasibility of chlamydia vaccine depends on producing a protective host defense which may include S-IgA response, a cell mediated response and possibly a humoral antibody. In addition, the ability to produce large quantities of this antigen indicates a synthetic and/or chimeric antigen may be the method of choice.
Idiotypes have been intensively studied following Jeme's network theory in 1974. One of his major proposals is the self regulation of the immune system through a network of idiotype-anti-idiotype interactions (Jeme, 1974). it is sug-gested that the idiotopes on a single antibody molecule can mimic ( that is, be the "internal image") of any foreign or self epitope at the molecular level.
All idiotypes of a single immunoglobulin molecule have been found to be located on Fv (fragment variable) region by studies showing that the inhibition of binding of anti-idotypic antibodies to the idiotype is the same between Fv and Fab( Givol, 1991). In general, anti-idotypic antibodies are divided into three types Ab2 a , Ab2 a and Abas. Only Ab2 ~3 binds to the complementary determining region, thus can be the internal image of the antigen. The occurrence of Abz displaying internal image of properties must adhere to the following criteria;
(1 ) binding onto Abp and to any other anti-nominal antigen antibodies from another species and lack of reactivity with Ab2 to other antibodies; (2) inhibition of the binding of Ab, to the specific antigen, the nominal antigen, and (3) the ability to elicit the synthesis of Ab3 with anti-antigen specificity in animals without previous exposure to the antigen (Ertl and Bona, 1988).
The important role of anti-idiotypic antibodies in vivo has been shown in numerous experiments. The administration of anti-idiotypic antibodies was found to elicit different effects: either suppression or enhancement of the responses to the specific idiotype( Hart, 1972, Kennedy, 1983). In autoirnmunity, it certainly plays an important role. The pathology associated with many autoimmune diseases is most likely due to (at feast in part), a direct idiotype-anti-idiotype interaction of the autoimmune antibodies with anti-idiotypic antibodies.
Idiotypic specificity in a specific antibody were first characteri2ed, by demonstrating that specific hapten binding could inhibit idiotype recognition. The first experimental support for the validity of the internal image was presented by Sege and Peterson in 1978 by using anti-idiotype as a probe to identify cell surface receptors.
The best information for the exact molecular basis for the mimicking presently is obtained from the X-ray crystallography of the idiotype-anti-idiotype complex. The basis of molecular mimicry of the antibodies can be either local sequence homology to the original protein as in a reovirus system or, in most cases, identical conformations from entirely difFerent amino acid sequences as in the hemoglobin-myoglobin family of proteins. X-ray crystallography and seruence data in the later studies showed that identical, functional conformations can be assumed by proteins that differ by as many as 137 of 141 amino acids. The studies of the crystal structure of idiotope-anti-idiotope complex in the anti-lysozyme antibody and the anti-idiotope have demonstrated that a private idiotope consists of 13 amino-acid residues, most from the complementarity-determining regions, but including three residues from the third framework region of its VL domain. Seven of these residues are common with the paratope of anti-lysozyme antibody, indicating a significant overlap between idiotope and antigen-combining site. Idiotype has been a unique tool in characterization and manipu-lation of the immune response since it was found and realized: as a clonal marker to follow B cell development, somatic mutation and fate of clones of B
cells. They have been used as a phenotypic marker for germ-line V genes.
Anti-idiotypic antibodies which bear the internal image of external pathogens such as virus, bacteria or parasites have been used as surrogate antigens for vaccine and are being used in treating B cell lymphoma and autoimmune disease such as encephalomyelitis. In addition, it has been shown that anti-idiotypic antibodies can induce T-cell responses in which either by toxic T-cells or T-helper cells are produced which recognizes the original antigen.
' 11 Since chlamydia are intracellular parasites, current tests emphasize the importance of collecting cellular material from the specimen to be tested.
When utilizing these tests, an extraction method is required in order to separate the chlamydial antigen from the cellular material when an immunological test is performed. Thus, presently available diagnostic tests for chlamydia are based upon detecting the presence of major outer membrane protein (MOMP) or iipopolysaccharide (LPS). The presently available diagnostic procedures for MOMP are undesirable since they lack sensitivity and specificity. Diagnostic tests based upon LPS are undesirable since LPS is present only in small amounts and the procedures needed to concentrate LPS are complex. In addition, diagnostic tests based upon cellular material are undesirable since they require culturing of cells which is time consuming and they require processing of cellular material which is time consuming and complex.
It has also been proposed in Current Microbiology, Vol. 28, pages 85-90, 1994 to provide a diagnostic test for cells infected with chlamydia based upon the production of GLXA from cultured cells infected with chlamydia. While the disclosed assay method for GLXA was shown to be useful for assaying for GLXA
obtained from cell cultures, no determination has been made that the assay method is useful for assaying GLXA in bodily fluids such as urine or serum.
While the diagnosis for the presence of GLXA antibodies in a bodily fluid is useful to determine whether an animal or a human has been previously infected with chlamydia, it is not useful to determine whether the animal or human is infected with chlamydia at the time of diagnosis.
Accordingly, it would be desirable to provide a diagnostic test for chlamydia which is specific and sensitive. In addition, it would be desirable to provide such a diagnostic test which is suitable for all serovars of chlamydia.
Furthermore, it would be desirable to provide such a test which is specific and sensitive to an antigen of chlamydia which can be found in extraceilular biological fluids of animals and humans which does not require lysing of cells. Such a test would eliminate the need to culture or otherwise process cells.
In one aspect, the invention provides a method for immunochemically diagnosing Chlamydia in a mammal which method comprises: contacting an extracellular biological fluid from said mammal with antibody specific for a genus-specific Chlamydial glycolipid exoantigen; measuring any specific binding immunocomplexes formed between the antibody and any Chlamydial glycolipid exoantigen present in the fluid; and comparing the amount of the immunocomplexes formed in the fluid with the amount of immunocomplexes formed by a control fluid from a mammal free of Chlamydia infection, wherein a greater amount of immunocomplexes in the fluid than that found in the control fluid indicates the presence of Chlamydia infection in the mammal.

BRIEF DESCRIPTION OF THJE FIGURES
Figure 1 is a binding curve of guinea p~ antisera to monoclonal GLXA
Abp.
Figure 2 is a binding curve of guinea pig anti-monoclonal GLXA Ab, IgG
antisera to normal mouse IgG before and after immunosorption.
Figure 3 is a curve showing the inhibition of the binding of monoclonal GLXA Ab, to Gi~CA by absorbed guinea pig anti-idiotypic antisera.
Figure 4 is a curve showing fractionat'ron of guinea pig anti-idiotypic IgG.
Figure 5 is a curve showing the inhibition of the binding of monoclonal GUCA-AB, to GLXA by guinea pig anti-idiotypic isotypes.
Figure 6 is a curve showing the binding of rabbit anti-anti-idiotypic antibody to guinea pig anti-idiotypic IgG.
Figure 7 is a curve showing the inhibition of the binding of monoclonal GIxA Ab, to GLXA by rabbit GLXA-Aba.
Figure 8 is a curve showing the detection of chlamydial spedfic ribosomal RNA from primates.
Figure 9 is a curve showing the effect of GLXA Ab, IgG on ocular infection by clinical disease score.
Figure 10 is a curve showing the inhibition of binding of monoclonal GLXA
Ab,, to GLXA by a hybridoma done.
Figure 11 is a curve showing the direct binding of chlamydia patient antiserum to monoclonal GLXA-M Abz.
Figure 12 is a curve showing that rabbit anti-chlamydia antiserum recog-nines monoclonal GLXA-M Abz.
Figure 13 is a curve showing the protection of mice from chlamydiai infection by immunization with monoclonal GLXA-M Ab2.
Figure 14 is a protection curve by monoclonal GLXA-M Ab2 igG after a high dose of ocular infections.
13a Figure 15 is a curve showing the effect of alum on the protection of mouse chlamydial inf~ion.
Figures 16 A and B show curves of the time course of ocular infec~ivity after immunization with monoclonal GL.X~Ab2.
SUMMARY OF THE INVENTION
The present invention is based upon the discovery that a diagnostic test for the presence of chiamydia in a human or an animal can be efPec~ed with a extracellular biological fluid of the human or animal such as urine, tears, saliva, nasal phargyniai fluid, cervical swab fluid or vaginal swab fluid. The extraoellular biological fluid is tested for the presence of GLXA with the idiotypic antibody to GLXA (hereinafter GIxA Ab, ) or the anti-anti-idiotypic antibody (hereinafter GLXA-Abp ) which is the antibody to the anti-idiotypic antibody to GLXA Ab, (hereinafter GLXA Abz ). In accordance with this invention, it has been found that an extracellular biological fluid obtained directly from the human or animal can be assayed for the presence of GLXA which is a sensitive and specific marker for all known forms of chlamydia. The diagnostic use of this invention can be utilized in any of a variety of modes including direct assay,indirect assay, competition assay or sandwich assay. Thus, the diagnostic test of this inventron provides substantial advantages over prior art tests which requins cellular material from the human or animal being tested.
DESCRIPTION OF SPECIFIC EMBODIMENTS
The Gt.XA is obtained and purfied by any presently available method.
Thus GLXA can be isolated on an octylsepharose column and eluted with alcohol or isolated on DEAF Sepharose and eluted in low pH aqueous solution or isolated on a polyacrylamide bead column and eluted with low pH aqueous solution of KSCN. (5M). In a preferred method GLXA is obtained arid purified from supernatant of infected cell cultun~s.by presently available methods such as by exclusion chromatography over a Sepharose 68-CI column in 0.075 M
phosphate, 0.154 M NaCI, pH 7.2. The GLXA appears in the front fraction of the *Trade-mark column and is detected by a chemiluminescence assay using an acridinium ester conjugated monoclonal GLXA-Ab,. The fractions containing the GLXA are usually contaminated by nucleic acids, but not protein. The GIxA fractions are pooled, concentrated and treated with RNase and DNAase at pH 8.0 for about 2 hours at 37° C. The mixture is rechromatographed over the same column and is now pure. It can be stored at 4° C (with or without preservative).
The antibody can be polyclonal or monoclonal. In the production of monoclonal antibody, an idiotypic antibody GLXA-Ab, is provided by immunizing an animal, usually a mouse, with GLXA or the chlamydia bacteria as the antigen.
Immune spleen cells of the animal then are identified, isolated and fused with lymphoma or myeloma cells by being contacted with a fusing agent such as polyethylene glycol such as by the procedure of Kohler & Milstein, Nature 256:
459, 1975. The fused cells then are incubated in a selective medium such as HAT medium which precludes the growth of unfused malignant cells. The hybridoma cells are cloned by limiting dilution and supernatants are assayed for secreted monoclonal antibody of desired specificity. A suitable hybridoma for producing GLXA-Ab, is deposited in the American Type Culture Collection and identified as ATCC H.B.11300. Monoclonal antibodies also can be obtained by ascitic growth of hybridomas in vivo. Alternatively, the lymphocyte cells can 'be immortalized by exposure to Epstein-Barr virus. The idiotype antibody, GLXA-Ab, is useful in producing GLXA-Ab2 which, surprisingly is active in immunizing against or neutralizing a chlamydia infection. In addition, GLXA-Ab2 is not species specific but is genus speck in that its immunization and neutralization activity is useful in many animal species. The monoclonal Gt~CA-Ab2 also can be produced by the process utilizing hybridorrias set forth above for GLXA Ab, but by utilizing GLXA-Ab, as the antigen. A suitable hybridoma for producing Gt~CA-Ab2 is deposited in the American Type Culture Collection and identified as ATCC
_ H.B.11301. GIxA-Abp also can be produced as a polyclonal antibody and, as a polyclonal antibody it is active for immunization against or neutralization of infection by chlamydia. Polyclonal antibodies are made in any conventional manner wherein a first animal is immunized with GLXA as the antigen and polyclonal GLXA-Ab, is isolated from the animal's serum. The polyclonal GLXA-Ab, or monoclonal GLXA Ab ~, then is injected into a second animal of a different -species from the first animal and polyclonal GLXA-Ab2 then is recovered from the second animal's serum.
Any conventional test procedure can be utilized in the present invention including radioimmunoassay, enzyme-linked immunosorbent assay, fluorescent assay, chemiluminescent assay, competitive immunoassay, membrane-based immunoassay, precipitation, agglutination, antigen capture or the like.
While the present invention can be utilized to directly test extracellular biological fluids, it is to be understood that the present invention also is useful for testing for chlamydia in cells obtained from a human or animal wherein the presence of GLXA can be determined. However, it is preferred to test an ex-tracellular biological fluid since the manipulative steps needed to effect the assay are less complex than with samples having cells which are lysed.
The labeled antibody Ab, or Ab3 or Fab fragment thereof can be utilized to interact directly with the extracellular biological sample to form a bound complex with any GLXA present in the sample. The concentration of GLXA present in the sample is determined by measuring the concentration of the detectable label in the antigen (GLXA)-antibody complex formed, if any. Alternatively, the con-centration of GLXA can be determined with a conventional competitive assay wherein the Ab, or Ab3 -based antibody can interact either with an unknown concentration of GLXA and a known concentration of Ab2 or Fab fragment of Ab2 The concentration of GLXA in a sample also can be determined indirectly with labeled Ab2 or a ~Fab fragment of Ab2. In this procedure, any GLXA present is first complexed with Ab, or Ab3 of Fab fragment thereof. The labeled Ab2 or Fab fragment thereof then is interacted with the complex to form a second complex containing the detectable label.
16 ' A preferred diagnostic procedure is:
Direct Sandwich Assay Where immobilized Ab, or Ab3 or Fab fragment thereof captures any GLXA
- present in the sample of extracellular biological fluid. The concentration of bound GLXA is then determined by interaction of labeled Ab, or Ab3 or Fab fragment thereof and measurement of the detectable label in the antigen (GLXA)-antibody complex formed, if any.
The following examples illustrate the present invention and are not intended to limit the same.
Example 1 Throughout this study, two serovars of C. trachomatis were used. Serovar B (Strain Har 36) organisms originally isolated from conjunctiva) scraping of a child, were grown at 37°' C on McCoy cell monolayer with Eagle's Minimum Essential Medium with Hank's. balanced salt solution (HMEM, Whittaker, MD) and stored at -70° C in the same medium with 10% of dimethyl sulfoxide (Sigma Chemical Co., MO). Serovar C (TW-3) was grown in mass tissue culture in McCoy cells. The elementary bodies were purified by centrifugation through renograffin and resuspended in phosphate-buffered saline and stored at -70° C.
Chlamydia free Hartley strain inbred guinea pigs were originally obtained from Jackson Laboratory (Bar Harbor, ME), bred and maintained in an animal facility. One year old females were used in this study.
Female New Zealand rabbits free of Pasteurella were obtained from Mill Broock Farm (Hadly, MA). The rabbits were about 6-8 pounds when received and used within one week. BALB/c ByJ (H-2d) mice were obtained from Jackson Laboratory (Bar Harbor, ME). Young adult cynomolgus monkeys (Macacca fasicularis) were obtained from Charles River Primates, Inc. (Port Washington, NY) which were free of clinical ocular diseases. All the primates had been used for a previous ocular infection with C. trachomatis serovar C elementary bodies, some primates had been previously immunized with a chlamydial protein. The primates challenged at this study, were free of the disease and were not im-mune. They were randominized prior to the initiation of the experiment. All procedures were performed under anesthesia.
Production of Polyclonal Anti-idiotypic Antibodies For the production of polyclonal anti-idiotypic antibodies, each of six guinea pigs was immunized subcutaneously with 150 ug of monoclonal GLXA- ' Ab, (89MS30) IgG in 1 ml of H20 plus 1 ml Maalox Plus suspension ~(liam H.
Roger, Inc., PA). Three weeks later the guinea pigs were boosted with 100 ug of monoclonal GLXA-Ab, in 1 ml of Maalox (aluminum hydroxide, alum) and H20, and were boosted on a monthly basis.
For the production of anti-anti-idiotypic antibodies, three rabbits were immunized with absorbed anti-idiotypic guinea pig isotype IgG-I, 300 ug in 1 ml of alum and 1 ml of H20 intradermally on multiple sites and boosted three weeks later using the identical protocol. Subsequently, rabbits were boosted at monthly intervals. For the production of monoclonal anti-idiotypic antibody, GLXA-Ab2 {91 MS441 ), fifty ug of KLH conjugated monoclonal GLXA-Ab, IgG was injected into five 9-week old female BALB/cByJ mice intraperitoneally in an equal amount of complete Freund's adjuvant (Sigma, MO). The same amount was used in the subsequent booster at day 14 and later on a weekly basis for five weeks in the presence of incomplete Freund adjuvant. A final booster injection was given 3 days before the removal of the spleen.
Monoclonal GLXA Ab, IgG was isolated by protein A affinity chromatog-raphy. The ascites which contains monoclonal GLXA-Ab, IgG was first centri-fuged 2000 rpm for 10 minutes at 4° C and passed through glass wool to remove lipids and precipitates. The affinity column (1.5 x 9 cm) packed with 2 ml Protein A Sepharose CL4B (ZYMED, CA) was first equilibrated in a binding buffer (1.5M
glycine, 3M NaCI, pH 8.9) (Jackson lmmunoResearch Laboratories, PA). Two ml ascites diluted with equal amount of binding buffer was loaded onto the column at 0.6-0.8 ml/minute. The column was stopped for about 30 minutes to allow banding and then rinsed with about three bed volumes of binding buffer. The bound IgG was eluted with 0.1 M citric acid, pH 3, into glass tubes which contained 50 ul 0.1 M TBS, pH 8.0 to equilibrate the pH. IgG was detected by an atsorption at 280 nm. The absorption larger than 0.1 was pooted,and dialyzed against 0.075 M PBS, pH 7.2 overnight. The purity of the IgG isolated was confirmed by SDS PAGE on a PhastSystem* (Phamacia, NJ).
The specific response of guinea pig immunized with monoclonal Ab, IgG
was detected by direct enryme-linked immunosorbent assay. A 9fi well plate with Immulon~2 removable strips (Dynatech, RI) was coated with 0.4 ug of monoclonal Ab, tgG per well in coating buffer (0.015M NaHCO~, 0.3M glycine, 0.02% NaN3 with 0.06M polyethylene glycol, PEG), pH 8.6. The plate was stored at 4° G
overnight. Each plate was rinsed three times with 0.05% Tween 20 in 0.075M
PBS and blocked with 1 % BSAIPBS for 2 hours at room temperature. Again, the ptate was rinsed three times. The pre-immune sera or antisera from guinea pigs were serially diluted with 0.075M PBS and 100 ul of each was added to each well in duplicate. The mixture was incubated at room temperature for 1 hour and rinsed. Goat anti-guinea pig IgG (H & L) horseradish peroxidase conjugate (Jackson immunoResearch Labs, Inc. PA) 1:1000 was added, incubated for one hour and rinsed. TMB substrate (Kirkegaard and Peny Laboratories, MD) was added after rinsing. The absorbance at 405 nm was determined using a Vmax microwell reader (Molecular Devices Corp., CA). The antisera from rabbits immunized with guinea pig IgG-1 was assayed in the similar manner. Each plate was coated with guinea pig IgG-1 and the second antibody was goat anti-rabbit (H and L) horseradish peroxidase conjugate (Jackson Immune Research Labs.
Inc., PA).
Normal mouse IgG (Jackson ImmunoResearch Labs Inc., PA) was conjugated to Affi-Gel 10 (Bio-Rad Laboratories, CA) as indicated by the manu-facturer. Briefly, 5 ml Affi-Gel 10 slurry was transferred to a glass fitted funnel connected to an aspirator and washed ~ with three bed volumes of isopropyl *Trade-mark alcoaol followed by three bed volumes of ice cold deionized water. Normal mouse 1gG (5 mg/ml), 10 ml was mixed with Aff~-Gei~lO in a vial. The coupling was done at 4° C overnight with gentle end to-end agitation. A column (0.9 x 5mn was packed with the coupled gel and rinsed with. 0.075M PBS, pH 7.2. The W absorbanoe at 280 nm of the effluent was monitored. The highest abso~
bance of this portion was used to test for protein content by the Bradford Assay (Bio-Rad Laboratories, ~ CAj to evaluate the conjugation.
A pool of one guinea pig antisera 3, 4 and 5 weeks after the immunization was absorbed by affinity chromatography on a nom~al mouse IgG-agarose column. The column was prepared as above. The antisera, about one void volume, was loaded onto the column and incubated for 30 minutes at 4' C and eluted with 0.075M PBS, pH 7.2. The antiserum was absorbed a second time with a freshly prepared column.
Five mt of guinea pig antisera which had been absorbed by normal mouse IgG, was loaded onto a protein A conjugated sepharose column, and rinsed with 0.02M phosphate-citrate buffer, pH 7.3. Guinea pig immunoglobulin subclasses IgG-1 and IgG-2 were eluted separately using a step pH gradient of 4.9 until no protein was detected in the effluent. The ~iumn was then eluted with a low pH
gradient, 4.3. After djalysis against 0.02 M phosphate-citrate buffer, pH 7.3, each isotype was subjected to a second round of subclass separation.
Production and Characterization of Monoclonal Anti-idiotypic Antibodies (monoclonal GLXA~Ibz) Monoclonal Abp (89MS30) IgG was isolated from a protein A chromafio-graphy column as set forth above. The keyhole limpet hemocyanin conjugation was carried out by using glutaraldehyde. Briefly, 1.5 mg of IgG was mixed with 0.05 mg KLH, (Sigma Chemical Co., MO) (approximately 1 molar of IgG per 50 amino add of KLH) in equal volume of 0.2 °~6 of glutaraldehyde in PBS, in-cubated at room temperature with gentle stirring. One hour later, i M of glydne was added to make a final concentration of 0.02M and incubated for another *Trade-mark 20 hour ai room temperature. The conjugate was then dialyzed against PBS
overnight.
Four days after the last boost (see immunization), spleen cells were isolated from two mice which had the highest titer. Fusion was made with mouse myeloma cell tine Sp 2/0-Ag14 according to the technigues initially develped by Kohler and Milstein (Nature, 1975) and modified (Goldsby, A practical Guide to Making Hybridomas in Nucleic Acid & Monoclonal Antibody Probes, Swaminathn & Prokask, Eds. Deller. N.Y. pg. 367, 1989). Feeder cell layers were from spleens of mice 8 weeks old.
Anti-idiotypic antisera from immunized mice and supernatants from cloned cells were detected by a sandwich ELISA (Uytdehaag et al, J. Immunol. 134:
1225, 1985, Hiroshima et al, J. Immunol. 144: 224, 1990). Briefly, polystyrene Immulon II microtiter plates (Dynatech Laboratories, Inc., VA) were coated with 100 ul of 1 ug monoclonal Ab, IgG in 0.1 M carbonate buffer, pH 8.9 overnight at 4° C. The unbound IgG was removed and the wells were blocked by 3%
BSA/PBS for 1 hour at 37° C. After washing, serial diluted antisera or 100 ul of culture supernatant from wells with hybridoma cells was added. After 1 hour incubation at 37° C and washing, 1 ug of biotin conjugated monoclonal Ab, IgG
was added to each well and the reactivity was detected by the addition of streptavidin-horse-radish peroxidase (Jackson Immune Research Labs., PA).
One hour later, TMB peroxidase substrate (Kirferggaard & Perry laboratories, Inc., MD) was added. The absorbance was read at 405 nm in a microplate reader. As positive and negative controls, immune sera taken before the fusion (1:10 dilution) and medium alone were used.
The inhibition of the binding of monclonal GLXA-Ab, to GLXA by mouse antiserum and the supernatant of the clones was determined by immune-chemi-luminmetric assay as described above.
Ten BALBlcByJ mice were injected with pristane (2,6,10,14-tetra-methylpentadecane, Sigma Chemical Co., MO), 1 ml per mouse intraperitoneally.

Ten days later, the mice were injected with approximately 2x106 monodonal GLXA Ab? (91 MS441) producing hybridoma cells. The asdtes was harvested by using a Vacutainer 20 G blood collection needle (Becton Dickinson, NJ.) about ten days later. The ascites was clarified by centrifugation, 2000 rpm for 10 minutes arid stored at -20° C until use.
The isotyping was carried out by ELISA. The supernatant from done 91 MS441, (100 ul), was coated in each well and incubated at 4° C
overnight. After rinsing and blocking with 3% BSA/PBS for 2 hours, 100 ul of rabbit antisenrm specific to mouse subclass: IgGi, IgG2a, IgG2b, IgG3, IgM, IgA, K chain or a chain (Bio-Rad Laboratories, CAA) was added to each well in duplicate. The plate was incubated at room temperature for one hour. The rabbit antiserum was detected by horseradish peroxidase conjugated goat anti-rabbit (H' and L) and TMB substrate (Kirkergaard 8~ Perry Laboratories, inc. MD).
The monoclonal GLXA-Ab2 IgG was purfied by affinity chromatography on a protein-G-sepharose column. Protein G-Sepharose~'4B (Zymed, CA) (5 mn was packed in a 0.5 x 9 cm column. The ascites {2 ml) was diluted 1:1 with 0.02M phosphate buffer, pH 7.3 and loaded on the column and washed with the same buffer until no protein was detected. The bound IgG was eluted with 0.1 M
dtric-glycine buffer, pH 2.8. The eluent was collected in 1 ml fraction which contained 50 ul of 1 M tris-saline buffer, pH 8Ø Fractions having W
absorption above 0.1 were pooled and dialyzed in PBS overnight at 4° C. The purified IgG
was identified by SDS-PAGE for confirmation.
Polyclonal antibodies from a human patient diagnosed with a chlamydial infection and chlamydial EBs injected rabbits were tested for the recognition of monoclonal GLXA Ab2 by ELISA. The procedure was essentially the same as described above with the following exceptions. Briefly, the EL1SA plate was coated with 1 ug of monclonal GLXA Ab2 per well in 0.075M PBS without coating buffer overnight at 4° C. The wells were rinsed with 0.05% Tween 20 in 0.075M
PBS and blocked with 3~o BSAIPBS for 2 hours at room temperature. Serial *Trade-mark WO 96/29604 PC'TlUS96/02617 dilution of tire patient's serum (92MS273), control human serum (88MS356), rabbit antisera (88MS188) or control, rabbit serum (92MS450), 100 ul, was added to each well in duplicate. After 1 hour incubation at room temperature, the wells were washed 3 times and 100 ul of peroxidase conjugated goat anti-human or goat anti-rabbit IgG (Jackson fmmunoResearch Labs, MD) was added. TMB
substrate was added after one hour incubation. The plate was read on a Vmax microplate reader (Molecular Devices Corp., CA).
Immune-dot blot assay was done by the same .method as described above. The exception is that a PVDF sheet was coated with purified GLXA (100 ul) per lane in 0.075M PBS. Antisera taken from the mice which were immu-nized with monoclonal GLXA-Ab2 IgG or normal mouse IgG were serially diluted with 3% BSA/PBS. The second antibody was horseradish peroxidase conjugated rabbit anti-mouse IgG (H and L). The photograph was taken by Kodak TMAX
100. The staining intensity of dot blot was scanned by a densitometer.
Production of Antigen C. trachomatis serovar B (Har. 36) elementary bodies were propagated in a McCoy cell monolayer in a 2 liter roller bottle (Corning, PA) in HMEM with added L-glutamine (final concentration 0.5 mM), NaHC03 (final concentration 0.4 mM) and 10 % of fetal bovine sera (FBS). Briefly, the medium was removed from the bottle after confluence of the monolayer. Then, 0.5-3.0 ml of EBs suspension (depending on the density of the organisms) in 40 ml of cycloheximide overlay medium (COM) (Whittacker, MD) with added L-glutamine and FBS was inocu-lated and the bottle was rolled at 3 rpm at 35' C. Two hours later, 20U ml of COM was added and rolling continued for 48 to 72 hours. The supernatant was obtained -after centrifugation to remove organisms and any cell debris.
GLXA was purified by two steps from the supernatant. First, the super-_ natant was passed though an octyl-sepharose CL4B column and eluted with 95%
ethanol (Stuart and MacDonald, Current Microbiology, 11:123, 1984). The antigen in ethanol (antigen content equivalent to 50 ml heavily infected tissue culture supernatant) was concentrated to approximately 50 ul and resuspended in 0.1 M phosphate buffer, pH 7.5. to i ml. Second, antigen thus prepared was further purified k,y afFinity chromatography. The affinity column was prepared by ' conjugating monoclonal GLXA-Ab, IgG to Affi-Gel 10 (Bio-Rad Laboratories, CA) as instructed by the manufacturer. The sample was centrifuged and loaded on to the affinity column and incubated for 30 minutes at 4' C. The column was rinsed with 0.1 M phosphate buffer until the eluant became clear. GLXA was eluted in 5M of potassium thiocyanate (KSCN, Mallinckrodt Inc., KY) with about 15-20 ml and dialyzed against 0.075M PBS overnight.
GtXA used in the immune-dot blot assay of binding of GLXA and monoclonal GLXA-Ab2 by GLXA-Ab3 described below was isolated by a size exclusion method. Sepharose CL-CB column (2x100 cm) was equilibrated with 0.075M PBS. The supernatant from C. trachomatis serovar F cell culture was first centrifuged 5000 rpm to remove cell debris and approximately 20 ml was loaded onto the column. The flow rate was 0.5 ml/minute. GLXA in the eluant was detected with Magic Lite Analyzer (Ciba Corning Diagnostic Corp., MA). The protocol is as described as below.
Inhibition of the binding of monoclonal GLXA-Ab, 1gG to GLXA by guinea pig GLXA Abz or rabbit GLXA-Ab3 (antisera, IgG, IgG isotypes) was detected by chemiluminometric immunoassay with a Magic Lite Analyzer (Ciba Corning Diagnostic Corp., MA). The protocol for the inhibition was as follows:
Affinity purified GLXA was diluted 1:5 with reagent A (Ciba Corning), mixed and ali-quoted into plastic tubes (200 ulltube, Sarstadt, NJ). A neutralizing solution Reagent B (Ciba Corning), (100) ul was added to each tube and mixed well.
Serial dilutions of guinea pig GLXA-Ab2 or rabbit GLXA-Ab3 IgG, (50 ul) were added to each of the above tubes and incubated at room temperature. One hour after the incubatio~~, 100 ul acridium ester-labeled (AE-labeled) monoclonal GLXA Ab, igG in 1 % BSA/PBS (befinreen 220,000 to 240,000 relative light units, RLU) was added into the mixture and incubated for one hour. Then, polyclonal anti-chlamydial antibodies which were covalently bound to paramagnetic particles (500 ul) was added to each tube and incubated for another hour. The bound immune complex (paramagnetic particles-GLXA-GLXA-Ab , AE labelled mono-clonal GLXA-Ab, IgG) is separated from the unbound by subjecting the mixture to a riiagnetic field. The particles were rinsed 3 times. Bound AE-labeled antibody was measured by the Magic Lite Analyzer and RLU were recorded. The percent-age of inhibition of binding was calculated as follows:
Inhibition =RLU control -RLU test X 100 RLU control where control represents PBS and test represents either pre-immune or antisera (or IgG) added respectively.
A Bio-rad dot blot apparatus was used for a direct assay. Poly-vinylidene fluoride (PVDF) membrane, 0.45 um, Immobilon-NC (Millipore, MA ) was coated with the affinity-purified GLXA or chlamydial rLPS for 18 hours at 4°
C. The membrane was then washed with 0.05 % Tween 20 in 0.075M PBS
buffer, pH 7.2 and blocked for 2 hours at room temperature with 3 % BSA/PBS.
After rinsing, serial dilutions of rabbit GLXA-Ab3 IgG (90MS699) (isolated by protein A affinity chromatography, method see above) or monoclonal Ab, IgG
(89MS30) were added (100 ul per well), incubated at room temperature for 2 hours, and washed to remove unbound IgG. The PVDF sheet was removed from the apparatus and blocked with 3 % BSA/PBS for two hours with gentle agitation, then probed with 1:1000 dilution of peroxidase conjugated goat anti-rabbit IgG
(H
and L) or rabbit anti-mouse IgG (H and L) (Jackson ImmunoResearch Labs., PA) for 1 hour at room temperature. Unbound conjugated antibody was removed by washing in a petri dish for 4 times, 5 minutes with agitation. The binding was detected by 4 CN (4-chloro-I-naphthol) membrane peroxidase substrate system (Kirkegaard & Perry Laboratories inc., MD). Assays were carried out in duplicate.
Monoclonal .GL~:A-Ab, or rabbit GLXA-Ab3 IgGs were labeled with biotin. -Briefly, the GLXA-IgG was first dialyzed against 0.1 M sodium borate, pH 8.8 for 4 hours at 4° C. Then, 200 ug of biotinamidocaproate N-hydroxysuccinimide ester "
(Sigma Chemical Co., MO) per mg of IgG was added, and incubated at room temperature for 4 hours. Finally, 20 ul of 1 M NH4CI per 250 ul of ester was used and incubated for 10 minutes at room temperature to stop the reaction. Labeled IgGs were dialyzed against 0.075M PBS for 3 days at 4° C.
Confluent McCoy cell monolayers were grown on cover slips in a 24 well plate (Falcon, NJ) for 24 hours. The medium was removed from each well before 200 ul of C. trachomatis serovar B elementary bodies (Har 36) or 200 ul of HMEM alone were applied to each well. The inclusion forming units (IFU) was approximately 10001200 ul. Immediately after the application, 200 ul of cycioheximide overlay medium (COM) with L-glutamine and FBS was added to each well. The mixture was incubated at 37° C for two hours and the medium was replaced by 1 ml COM per well. The plates were then cultured for 48 hours at 37° C in a humidified incubator with 5% CO2.
After the incubation, cell cover slips were washed with 0.075M PBS twice, minutes each. The coverslips were then blotted with tissue carefully to remove buffer on the cover slips. Then 400 ul of 50 ug/ml biotin-labeled monoclonal GLXA-Abp or 400 ul of 1.20 mg/ml of biotin-labeled GLXA-Ab3 was added to the cover slips and incubated at 37° C for 1 hour. The cover slips were rinsed twice with PBS (five minutes each rinse). Four hundred ul of fluorescein-streptavidin 1:50 in 1 % of BSAIPBS was added and incubated for 1 hour. The unbounded fluorescein-streptavidin was removed as above. Fluorescence was detected by photograph with an Olympus 25, 35mm camera (ASA 400 TMAX black and white R'O 96/29604 PCTlUS96/02617 Kodak film) mounted on a Zeiss A.7082 Oberkichen microscope, illuminated with a 12v/IOOz halogen lamp.
Neutralization of Chlamydia by GtxA-Ab3 (90MS699) in vivo The rabbit pre-immune and GLXA-Ab3 IgG, normal mouse and monoclonal GLXA-Ab, IgG were filter sterilized. The IgGs (0.2 mg/ml) were mixed (1:1) respectively with C. trachomatis serovar C (TW 3) elementary bodies (200 in-clusion-forming units/20u1). The mixtures and non-treated EBs (as a control) were incubated at 37° C for 45 minutes, with gentle shaking every 15 minutes.
After the incubation, approximately 2 ug IgG plus 1000 IFU in 20 ul was inoculated onto inferior fornix of each eye of eight monkeys, four with GLX~,-Ab3 IgG plus EBs, two with pre-immune IgG plus EBs and two with EBs only. At the same time, 100 ul of each type of mixture was used to infect 10 wells of 2-day-old McCoy cell monolayer coverslip in a 48 well tissue culture plate for determination of the infectivity of the inoculum. Culture methods are described below.
Conjunctiva) swabs were taken by sweeping the interior tarsus and fornix, the lateral fornix, the superior tarsus and fornix, and the medial fornix on the day prior to inoculation, and on days 2, 6, 9, 13, and 20 after the inoculation.
The swabs were immediately immersed in 2 ml collection medium and disrupted by vortexing for 2 minutes in the collection medium.
Conjunctiva) swabs were first disrupted by vortexing for two minutes in the collection medium to collect EBs from the swabs. Then 200 ul of this collection medium was inoculated onto McCoy cell monolayer cover slips. The cells in a 48 well tissue culture plate were grown for two days, 5 wells for each sample.
For an in vitro neutralization experiment, 100 ul of the mixture was inoculated onto the monolayer cover slips of 10 wells for each sample. The inoculated plates were then centrifuged at 1,000 x g for 1 hour at room temperature. The plates were incubated at 3~° C for 2 hours and the medium was replaced by 1 ml of 10 % FBS in COM (Whittaker, MD). The plates were cultured at 37° C
in a humidified incubator with 5~/o C02. for 48 hours. The culture medium was aspir-ated from each well after the incubation. The monolayer coverslips were washed once with 0.075M PBS, fixed with ethanol for 5 minutes and then rinsed with twice. The fluorescein-labeled rabbit anti-chlamydial monoclonal antibody with Evans blue counterstain (Syva, Co., CA.) (25 ul) per well was added and in-cubated for 30 minutes at 37 °C. After the incubation, the wells were rinsed with H20 twice and a cover slip was mounted to each well with mounting fluid. The inclusion bodies were counted by inverting the plate on a fluorescence micro-scope.
The conjunctiva) swab (scraping) from each eye of infected primates was pressed on alcohol-precleaned glass slides. The slides were air dried and fixed with cold acetone for 5 minutes. Slides were then dried and 30 ul of fluorescein-labeled monoclonal antibody reagent with Evans blue counterstain (MicroTrak Chlamydia Direct Reagent, Syva Co. CA) were overlaid. The incubation was carried out in a covered, moist chamber. After 15 minutes, slides were turned on edge to remove excess stain and rinsed with deionized wafer for 10 seconds.
Slides were allowed to completely air dry. A cover slip was placed on each slide with mounting medium (Syva Co., CA) and sealed with fingernail polish. Slides were examined under a fluorescence microscope at 500x and 1250x. The infectious titer was scored on a semi-quantitative scale 0-4+: 0 is negative, 0.5 is negative on first passage and positive to any degree of second passage, 1 is for 1 to 9 inclusions per well on first passage and so on.

The clinical response of each eye was graded as ten clinical signs (Taylor et al, Invest. Opthalmol. Vis. Sci. 29:847, 1988): the follicular response in the lumbar, timbal, superior tarsal, superior fornix, and inferior fornix portion of the conjunctiva hyperemia or injection of the bulbar, superior tarsal, superior fornix, and inferior fomix conjunctiva and ocular discharge. The clinical response was graded on a scale of 0 to 3 for each of 10 signs of conjunctiva) inflammation to obtain a total inflammatory score for each monkey. The examiner was unaware about the allocation of the monkeys. The means of the scores were used to describe the response of a group of monkeys.
Total RNA was prepared from conjunctiva) swab samples taken from GLXA-Ab3 or normal rabbit IgG treated monkeys on the day before the challenge and on day 2, 6, 9, 12, and 20 after the challenge. The swab samples were first homogenized in phenol at 65% in the buffer containing 50 mM Tris (pH 8.0), 150 mM NaCI, 10 mM ethylenediaminetetraacetic acid (EDTA) and 1 % SDS. RNA
was precipitated and redissolved in the same buffer. This preparation of RNA
was extracted several times with phenol:chloroform (3:1 ), resuspended and treated extensively with DNase I. The quality of RNA preparation was monitored by ethidium bromide-UV visualization after separation on formaldehyde-agarose gels.
The probe used was a DNA fragment containing the 16S and 23S
ribosomal RNA and flanking sequences which was excised from the chlamydial genomic plasmid clone pL2, 434Sc1-IA (Cheema et al, The Amer. J. Med. Sci.
302:261-268, 1991). The DNA fragment was labelled by nick translation using s2PdCTP, 800 Cilm mole (Amersham Corp., IL). The specific activity for all restriction fragment probes was about 106 cpm/ug DNA. Slots on each blot included 1 ug of monkey or human-derived total RNA, 10 pg pure C. trachomatis or C serovar RNA (positive control), 3 ug yeast or rat RNA, buffer alone and 1 ug RNA from swabs of each monkey taken prior to infection (negative control). RNA

was fixed to 0.22 um filter (Schleicher and Schuell Corp., NH). The hybridization ' results were visualized via autoradiography at -70' C using X-OMAT AR film (Kodak, New York).
Inoculation and specimens C. trachomatis serovar C (TW 3) elementary bodies 5000/20u1 were inoculated onto each eye of the mice which were immunized with monoclonal Ab2 or normal mouse IgG. On the day before the inoculation and on day 7, 10, 14, 21, 28 and 35 after the inoculation, conjunctiva were swabbed from each eye.
The area included the inferior tarsus and fornix, the lateral fornix, the superior tarsus and fornix, and the medial fornix. The conjunctiva) swabs were immediate-iy immersed in the collection medium and disrupted for two minutes by vortex and kept on ice until culturing.
Detection and Characterization of Polyclonal Anti-idiotypic Antibodies The immunogen which was used to produce the anti-idiotypic antibodies in guinea pigs was a monoclonal antibody identified as 89MS30 (monoclonal GLXA-Ab, ). It was originally produced by immunization of BALBIcByJ mice with chlamydial elementary bodies propagated in embryotic egg. Mice spleenocytes ' were fused with Spa/0-Agl4 myeloma cells and the clone was screened. The clone (89MS30) reacted to all 15 serovars of C.trachomatis. C. pneumoniae, and C. osittaci 6BC and mouse meningopneumonitis by EIA, demonstrating recogni-tion of a genus specific antigen. The IgG was isotyped as IgG2b by ELISA using rabbit anti-mouse antiserum (Bio-Rad Laboratories, CA). The monoclonal GLXA-Ab tgG was isolated from the ascites with rec-protein A sepharose 4B conjugate column (ZYMED, CA). Inbred guinea pigs (Hartley 13) were immunized and boosted with monoclonal GLXA-Ab, IgG, 150 ug each in the presence of Maalox, as an adjuvant. Pre-immune sera and antisera were obtained by heart puncture and centrifugation. Five immunized guinea pigs demonstrated strong immune WO 96!29604 PCT/US96/02617 responses against monoclonal Ab, IgG by ELISA. It was demonstrated that the anti-monoclonal GLXA-Ab, !gG titer was more than 1 to 20,000 one week after the first boost. These guinea pig antisera kept increasing two weeks after the boost as shown in Figure 1.
In order to remove guinea pig anti-mouse antibodies that are directed against epitopes other than the idiotopes present on the hypervariable regions of the monoclonal Ab, IgG molecules, the guinea pig antisera was absorbed with normal mouse IgG. The absorption was carried out by affinity chromatography.
The column was made by conjugating normal mouse IgG to Affi-Gel 10. The conjugation was evaluated by detecting the amount of unbound protein at absorbance at 280 nm. The highest optical density from a fraction was 0.2;1, con-taining 0.18 mg of protein by the Bradford Assay (Bio-Rad Laboratories, CA).
The total mouse IgG used in the conjugation was 50 mg, demonstrating that the conjugation was successful. The guinea pig antisera were loaded onto the column and eluted with 0.075M PBS, pH 7.2. This procedure was repeated using a newly prepared column. The antisera before and after the absorption was tested and compared with pre-immune sera for the reactivity to normal mouse IgG by ELISA. The concentration of each antiserum for the assay was normal-ized. The result showed that sera after the absorption had the same reactivity against normal mouse 1gG as pre-immune sera (Fig. 2). The unabsorbed antisera had 5 times more reactivity, indicating that all antibodies specific to epitopes other than idiotypes have been completely removed.
If guinea pig antisera contain the specific anti-idiotypic antibody against monoclonal GLXA-Ab, IgG molecules, the direct effect is that it would inhibit the binding of antigen, GLXA, to the monoclonal antibody, monoclonal GLXA Ab,. In other words, the antisera bind to the complementarity-determining region of monoclonal GLXA-Ab, IgG, thus preventing GLXA from binding to the active site.
To test this, competition of binding was performed by chemiluminometric im-munoassay. Serial dilutions of guinea pig pre-immune sera, unabsorbed antisera, or absorbed antisera were incubated with GLXA which was isolated by immune-affinity chromatography. After one hour at room temperature, the mixtures were incubated with monoclonal GLXA-Abp IgG conjugated with acridium ester for an additional hour. Solid phase paramagnetic particles were added and a RLU was determined. As shown in Figure 3, when the guinea pig antisera was diluted 1:40, 95% of the binding of monoclonal Ab, to GLXA was inhibited by both unabsorbed and absorbed antisera, compared with 15 ~% for pre-immune serum.
in addition, the unabsorbed antisera had nearly identical inhibition as absorbed antisera at equivalent protein concentration, indicating that no anti-idiotypic antibodies were removed by absorption. Therefore, a competitive anti-idiotypic antibody had been generated in guinea pigs.
Previous experiments had shown that different isotypes of guinea pig anti-idiotype exert different effects on the idiotype production. IgG-1 isotype enhances the idiotype production, whereas IgG-2 isotype inhibits the idiotype clone. To test the inhibition of different isotype of guinea pig anti-idiotypic IgG, subclasses of IgG were isolated from absorbed guinea pig anti-idiotypic antisera. A step pH
gradient of phosphate-citrate buffer was used. IgG-1 and IgG-2 were separated and isolated on a protein A affinity column. The elution profile of the isotypes, IgG-1 and IgG-2 is shown in Figure 4. Each peak was identified by immuno-electrophoresis (IEP). Goat anti-guinea pig IgG (Bethyl, TX) was used to precipitate the bands. The first peak which is composed of IgG-1 formed a single band by goat anti-guinea pig antisera. The first peak was then repurified by the same method.
The competition by different subclasses of IgG was carried out again by chemiluminometric immunoassay using guinea pig anti-idiotypic antibodies of either IgG-1 or IgG-2 isotypes. Figure 5 shows that 0.4 ug IgG-I was able to inhibit the binding of monoclonal GLXA-Ab, to GLXA by 50 %. The total inhibition occurred when !00 ug was used. This was essentially tie same concentration needed when unlabeled monoclonal GLXA-Ab, IgG was used. IgG-2 showed little, if any, inhibition, approximately 25 % of the binding of monoclonal GLXA-Ab ~
to GLXA with L0 ug. These data demonstrate that the IgG-1 subclass of anti-idiotypic IgG was at least 5 times more inhibitory than the IgG-2 subclass.
The evidence obtained showed that guinea pig anti-idiotypic IgG-I was against the hypervariable region of monoclonal GLXA=Ab, IgG and also inhibited its binding to GLXA. The final criteria of an internal imaoe of the anti-idiotypic an-tibodies is to confirm structurally that the Ab2 is Ab2 /3 , not Ab2 a. Since Ab2 a binds to the framework portion of immunoglobulins, it can also inhibit the binding of Ab, to the cognate antigen. To confirm that guinea pig anti-idiotypic IgG-I
is Ab2, the isotype IgG-1 was used to produce an anti-anti-idiotypic antibody (GLXA-Ab3) which can recognize the GLXA epitope in an animal which has never been exposed to GLXA antigen, (Ertl et al,Proc. Natl. Acad. Sci. USA 81:2850, 1988). Three New Zealand white rabbits were immunized with guinea pig anti-idiotypic IgG-I in the presence of adjuvant, Maalox (alum). The antisera from one rabbit (S2) were tested against IgG-I by ELISA (Fig. 6). The titer increased with time after the immunization. The titer was much higher than 20,000 compared with pre-immune sera three weeks after the second immunization.
The dot blot apparatus (Bio-Rad Laboratories, CA) was used to detect the reactivity of rabbit antisera to GLXA. Antisera from two rabbits were tested.
Since monoclonal GLXA-Ab, is cross-reactive to chlamydial LPS, poiyvinylidene fluoride (PVDF) membrane was coated with both GLXA and chlamydial rLPS.
Both rabbits antisera recognized GLXA and LPS with high reactivity. When IgG
from rabbit (S2) (90MS699) was used, the dots were positive at a concentration of 0.006 ug per lane. Pre-immune IgG did not react. The IgG isolated from this antisera was tested for its capacity of inhibiting the binding of monoclonal GLXA-Ab, to GLXA, since GLXA-Ab3 produced by the internal image, GLXA-Ab2 should exhibit a similar binding. This is confirmed as shown in Figure 7. The inhibition by GLXA-Ab3 increases with concentration, but about five times less inhibitory compared to unlabeled monoclonal Ab,. This demonstrates that the guinea pig anti-idiotypic antibody IgG-I is the internal image of antigen, ULXA. GLXA-Ab3 IgG was further tested for the recognition of elementary bodies of C.
trachomatis in vitro.
Monoclonal GLXA-Ab, and GLXA-Ab3 IgG were conjugated with biotin by glutaldehyde. Labeled monoclonal GLXA-Ab, or GLXA-Ab3 was incubated with McCoy cell monolayer on coverslips which were infected with C. trachomatis serovar B (Har 36) elementary bodies for 48 hours. Non-infected monolayers were used as control. The florescence staining pattern of the elementary bodies by monoclonal GLXA-Ab, and polyclonal GLXA-Ab3 IgGs demonstrated that GLXA-Ab3 not only recognized the purified form, but also the native form of GLXA.
Neutralization of the Chlamydial Infection in Primates by GLXA-Ab3 IgG
(90MS699) The next question concerned the ability of monoclonal GLXA-Ab, or GLXA ~4b3 to neutralize chlamydia elementary bodies and thus protect host cells from infection. The experimental approaches utilized to answer this question involved neutralization of infection in cultured cells and neutralization of the infection in primate conjunctiva.
Neutralization in primate conjunctivae was determined by preincubating organisms with antibody IgG and detection of the effect on ocular infection.
The igG fraction of monoclonal GLXA-Ab, or Ab3 was incubated with elementary bodies of C. trachomatis serovar C. Normal mouse or rabbit pre-immune IgG as well as no immunoglobulin added served as controls. The mixture was inoculated to each eye of the primate. On the day before the and after the inoculation, con-junctiva) swabs were taken by sweeping different areas of the conjunctivae (see above). Ocular chlamydial infection in primates was determined by cell culture assay which included second-passage on days post-infection. As shown in Table 1, three primates were infected with monoclonal GLXA-Ab, treated EBs on the left eyes, GLXA-Ab3 treated EBs on the right. At the same time, two primates were infected with normal mouse IgG treated EBs (shown as NI ) or EBs alone on the left and right eyes alternatively. The same method applied to pre-immune rabbit IgG (shown as N3). All eyes inoculated with monoclonal GtxA-Ab ~ t~
Bated EBs were positive at least once (primate No. 515, 84, and 26). However, only one eye of the GLXA- Ab3 treated eye was positive once, at day 10 post-infec-tion, two of them were never positive (primate No. 515, 84 and 26). Eyes inoculated with normal mouse or pre-immune rabbit !gG treated EBs were all positive at least once (primate No. 563, 20, 17 and 329). The untreated EBs (shown as C) produced infection in two of the four eyes involved (primate No.
563, 20, 17 and 329). Although the data points are diminutive, they do show that monoclonal GLXA Ab, does not neutralize chlamydia in primate conjunctiva. On the other hand, it suggests that GLXA-Ab3 is neutralizing. In order to confirm that GLXA-Ab3 does neutralize, a number of tests were carried out, including: (A,) neutralization in cell culture (B), neutralization in primate conjunctiva (C), detec-tion by clinical culture assay (D), detection by direct fluorescence antibody cytology (E), chlamydia specific RNA probe hybridization and (F) determination of the severity of ocular infection by clinical scoring.

Table 1.

Neutralization of chlamydial infection in primate conjunctivae by Ab3 but not mAb, Primate Eye Ab DaY Following Infection 515 L mAb, - - + + -R pb3 _ _ _ _ _ R N, _ _ _ +

84 L mAb, - - - + +

R Ab3 - - - + -20 L N3 - - - + -R C - - - - -26 L mAb, - - + - -R Ab3 _ _ _ _ _ 17 L N, - - - + +

R C - - - + +

329 L C - - + - -R N3 - - - + +

'EBs treated with normal mouse IgG(N1), pre-immune rabbit IgG (N3) or EBs alone (C) were controls.
GLXA Ab3 neutralizes the chlamydial infection in vitro.
In vitro, cell culture assay was carried out with GLXA-Ab3 and pre-immune rabbit antibody. The pre-immune rabbit and GLXA-Ab3 (90MS699) IgGs were isolated by protein A affinity chromatography. The mixture of 10 ug of each IgG
and 100 ul serovar C EBs (1000 IFU/ml) or EBs alone were inoculated onto wells containing McCoy cell monolayers. Ten wells per sample were used. Inclusion bodies were detected by FlTC-conjugated monoclonal anti-chlamydiG antibody 48 hours after the incubation. IFUImI was based on 15 fields per well. As is shown in Table 2, Ab3 IgG reduced the infectivity 3 times higher compared to pre-' immune IgG, 5 times higher compared to EBs alone, indicating neutralization by GLXA-Ab3.
Table 2.
In vitro neutralization of chlamydial infection by Ab3 IgG
R~ trPatPC~ m~ith Mr~an IFl )/15 FiPlcic + ~ F M
Ab3 34.1 + 7.2 Normal IgG 93.8 + 22.4 None 155.3 + 5.5 GLXA-Ab3 neutralizes the chiamydial infection in primates Eight primates were randomly divided into three groups in this experiment. In the eyes, four primates received with purified EBs previously incubated with GLXA-Ab3 IgG (eight eyes), two received EBs previously incubated with pre-immune IgG
(four eyes) and two received untreated EBs (four eyes). On the examining day, the con-junctiva) swabs were taken and cell cultured. Since there is no significant differ-ences between the recipients of pre-immune IgG and EBs alone, the results are presented as 8 experimental eyes and 8 control eyes. Cell culture results are expressed as IFU/ml based on counting inclusions in 15 fields for two wells per sample. As shown in Table 3, 20 days after the challenge, 1 of eight eyes was positive compared to eight out of eight eyes that were positive in the control group.
When the accumulated results were examined, with GLXA-Ab3, 9 of 4Q (22.5%) were positive, in the contrast, 36 of 40 (90%) were positive without GLXA-Ab 3.

Table 3.
Neutralization of chlamydial infection in primate conjunctivae by Ab3 IgG by cell culture assays ay of No. of Eye Culture Positive Experiment Ab3 Preimmune Noneb Combined IgG Control 2 3/8 2/4 3l4 5/8 6 3/8 4/4 4l4 8/8 9 1l8 3/4 4/4 7/8 20 1 /R 4/4 4/4 R!R

a. Only one first passage negative sample was second-passage positive.
b. EBs were previously incubated without antibody.
In an parallel assay, direct fluorescence antibody cytology assay (DFA) was also carried out to evaluate the numbers of EBs from the conjunctiva) swabs.
The conjunctiva) swab samples were fixed onto slides and stained with FITC-labeled monoclonal antibody against C. trachomatis. It was considered to be positive when or more characteristic elementary bodies were seen on each slide (Micro Trak, Syva Co. CA). As shown in Table 4, EBs were detected in the GLXA Ab3 treated group on only two occasions, day 6 and 12 post-infection, while the remainder were positive through day 20. Only one eye was EB negative in the non-treated group at day 2, that was probably an artifact. EBs were detected in all eyes in this group for the remainder of the experiment. On the last examination day (day 20), none of the eyes treated with GLXA-Ab3 was positive, while 8 of 8 were positive in the combined control group. In addition, DFA and culture results are completely congruent.
Table 4.
Neutralization of chlamydial infection' by Ab3 using direct fluorescence antibody cytometry assay (DFA)a ' ay o , No. o ye a ture os~tive Experiment Ab3 Preimmune Noneb Combined IgG Control 0 0/8 0/4 ~ 0/4 0/8 20 fl/R 4/4 4/4 R/f3 was consi ere positive i s were oun on a s i e.
bEBs were considered previously incubated without antibody GLxA Ab3 substantially attenuates the chlamydial replication in conjunctiva) infection Chlamydial specific ribosomal RNA had been examined from those primate conjunctiva) swabs by a DNA probe (Cheema et al,The Ameri. J. Med. Sci.
302:261-268, 1991). Total RNA was extracted from conjunctiva) swabs taken from primate eyes. RNA from serovar C EBs, human or yeast were used as control. 32P-chlamydial DNA encoding ribosomal RNA16S and 23S genes was used to detect chlamydial specific RNA in a Northern slot-blot hybridization assay. As shown in Figure 8, control eyes (infected either with pre-immune rabbit IgG plus EBs or EBs alone) uniformly show significant levels of chlamydial RNA at all time points examined, similar RNA samples prepared from the eyes of GLXA-Ab3 treated organism show significantly attenuated levels of chlamydial RNA. This indicates that the neutralization happens at the very early stage of the infection.
The degree of conjunctival inflammation after inoculation with EBs pre-viously incubated with either GLXA-Ab3 or pre-immune !gG or without previous incubation was evaluated by clinical response. The clinical response was graded based on a total clinical disease scores (TCDS) derived from 10 clinical features of ' inflammation (Taylor et al, Invest. Opthalmol. mss. Sci. 29: 1847, 1988). The accumulative disease scores were obtained for each group of primates by examin-ing 10 signs existing in the conjunctiva. As shown in Figure 9, recipients of GLXA-Ab3 developed very little clinical disease and this declined after day 8.
Control animals continued to develop severe disease through day 21 post-challenge.
This pathological finding is consistent with cell culture, DFA and RNA
hybridization data.
Generation of And Characterization of Hybridoma Cell Lines Producing Anti-idiotypic Antibody.
Five syngeneic mice (BALB/cByJ) were immunized intraperitoneally with KLH conjugated monoclonal GLXA-Ab, IgG in the presence of Freund's complete adjuvant. The anti-idiotypic anti-sera against monoclonal GLXA-Ab, IgG from these mice were detected by sandwich ELISA. The titer was about 1:1000 three weeks after the immunization (data not shown). Fusions were made between Sp2/0-Agl4 cells and spleen cells from two mice which had the highest titer against monoclonal GLXA Ab,. The size of the spleens were almost twice the size of normal spleen. The clones were screened by the same method for mouse antisera testing. The pool of mice antisera or pre-immune sera diluted 1:10 was used as controls in all screening tests. Among 283 wells screened, 8 were considered positive against GLXA-mAb i with a titer two times or higher than negative control. These hybridomas were cloned. One clone (91 MS441 ) had the highest titer in ELISA and was propagated. The ascites was produced and IgG

WO 96/29604 PCTlUS96/02617 isolated. The isotype of IgG of this clone was identified to be IgGI, having a K light chain (Bio-Rad Laboratories, CA). The fusion results was summarized in Table 5.
Table 5.
Summary of fusion for anti-idiotypic antibodies Immunized Anti-id Titer Total Wells Wells Stable BALB/cByJ in with Positive of Cloned Anti-Mice Supernatant Growing Anti-id id Lines Hybridoma (%) ~ (% of Total) . 000 (2.8) (0.35) ig t c am:K eavy c am: g The supernatant from positive clones were further tested for the inhibition of the binding of monoclonal GLXA-Ab, to GLXA by chemiluminometric immuno-assay. Total inhibition of the binding was found from the supernatants of 4 clones without dilution. Two weeks later only one clone (91 MS441 ) was found stable.
As shown in Figure 10, at a dilution of 1:10, the supernatant from this clone inhibits the binding of monoclonal GLXA-Ab, to GLXA by 80 % compared to 0% of a non-positive clone (91 MS442) from the same fusion. This demonstrates that an anti-idiotypic clone was produced. it is identified as monoclonal GLXA-Ab2.
As an internal image of an antigenic determinant, the anti-idiotypic antibody should be recognized by any specific antisera which is against this epitope regardless of species. In order to test this property of the IgG produce by clone (91 MS441), human serum from a patient clinically diagnosed as chlamydia positive was used. Since the isotype of monoclonal GLXA-Ab2 is IgGI, the purification of the IgG was carried out by protein G affinity chromatography. The isolated mono-clonal GLXA Ab2 IgG was coated on a microtiter plate and tested for reactivity with the patient's serum (91 MS253) by ELISA. Human serum without clinically diag-nosed chlamydial infection (88MS356) was used as a negative control. The results showed that the patient's serum had a titer which was more than 1:2000 against monoclonal GLXA-Abz (Fig. 11). This demonstrates that infected human antisera has the speck antibody against monoclonal GLXA-Ab2, implying that monoclonal GLXA-Ab2 is the internal image of GLXA.
The specific recognition of monoclonal GLXA Ab2 by a rabbit anti-chlamydial antisera (88MS188) was also tested in the similar way. The rabbit antiserum was produced by inoculating EBs. As shown in Figure 12, rabbit antisera has higher binding to monoclonal GLXA-Ab 2 than pre-immune serum, but lower than ex-pected. The difference between the binding is seen to the dilution factor of 1:1000. This shows that rabbit antiserum which is against chlamydia has the specific antibody recognizing monoclonal GLXA-Ab2, an additional evidence for monoclonal GLXA-Ab 2 as an internal image.
The anti-idiotypic antibody as an internal image can raise antigen specific antisera in animals that have never been exposed to that antigen. in this case, if monoclonal GLXA-Ab2 (91 MS441 ) is the internal image of GLXA, (that is bearing the same antigenic structure), it should produce an anti-GLXA antibody in the same strain BALB/c ByJ mice in spite of the fact that they have never been exposed to GLXA. In an initial experiment, 8 mice were immunized with mono-clonal Ab2 IgG, four mice with normal mouse IgG. No adjuvant was used in the subcutaneous infection. Seven days and 14 days after the immunization and one boost, antisera were obtained from these mice by sacrificing half of the mice in each group. Immune-dot blot assay was carried out with purified GLXA. The dot blot showed that mice immunized with monoclonal GLXA-Ab2 IgG had a titer as high as 1:800 compared to 1:100 or less of the mice immunized with normal mouse IgG. The blots were further quantified by a densitometer. When diluted to 1:900 after the first boost, the antisera from all four mice bind to GLXA
whereas no binding was seen in the control group even when diluted 1:50. This demonstrates .
that this antisera is solely elicited by the paratope of the anti-idiotype because the recipients are syngeneic.

W O 96!29604 PC iYUS96/OZ6I7 GLXA-Ab3 antisera which specifically bind to GLXA were also tested for the inhibition of the binding of monoclonal GLXA-Ab, by chemiluminometric im-munoassay. At a dilution of 1:25, GLXA-Ab3 inhibits 90% of the binding compared to 18 % of inhibition by the control antisera day 8 post immunization. This is equal to the same inhibition demonstrated by 10 ug of unlabeled monoclonal GLXA Ab,.
The same inhibition was found in the antisera on day 14, one week after the first boost with the same amount (50 ug/mouse) of IgG. !t is noted that inhibition percentage dropped from 70% on day 7 to about 50 % on day 14 when diluted 1:100.
immunization with Monoclonal GLXA-Ab2 Protects Mice from Chlamydial Infection BALBIc ByJ mice were used as an ocular chlamydial infection animal model in this study. The first experiment was carried out with 39 mice. Twenty mice were immunized subcutaneously with 50 ug of monoclonal GLXA-Ab2 and nineteen with normal mouse IgG without any adjuvant. They were given a total of three injections, one week apart. One week after the last injection, the mice were inoculated with C. trachomatis serovar C elementary bodies (5000 IFU in each eye). The conjunctiva) swabs were taken from each eye of the mice on day 0, 7, 14, and 21 post infection. Samples from conjunctiva) swabs were collected and cultured in McCoy cell monolayers for 48 hours. Inclusion bodies were counted, and 5 inclusions were considered as positive in 15 fields. As shown in Figure 13, mice immunized with monoclonal GLXA-Ab2 had half the infectivity compared with mice immunized with normal mouse IgG. In a second experiment (twenty mice in each group), the immunization was repeated in the similar manner. However, they received 106 IFU per eye, 100 times the number of EBs as used in the first experiment. Surprisingly, almost the same protection curve found in the mice (Fig.
14), suggesting that monoclonal GLXA-Ab2 elicits a vigorous host defense re-sponse.

!n a third experiment, aluminum hydroxide (alum) was used in the im-munization. Ten mice were immunized with monoclonal GI..XA-AbZ in the presence of adjuvant, eight mice immunized without adjuvant and s'acteen mice immunized with normal mouse igG in the presence of Maalox* The immunization procedure is the same as the previous ones. When Maalox was used in the immunization, the titer of the anti-anti-idiotypic antisera in mice was doubled as fiested against GL..XA
in immune-dot blot. The higher titered antisera in the adjuvant treated mice demonstrate more effective protection in the mice from the ocular infe~ion , compared to the ones immunized without alum (Fig. 15). However, nice irrr munized with monoclonal GI~CA~4b2 had significantly less infection than those receiving normal mouse IgG plus alum. In addition, the infection was cleared by post challenge day 28. In the fourth experiment, eight mice were immunized with monoclonal GLXA Ab2 and eight with normal mouse igG in the presence of alum.
The immunization and inoculation protocols are the same as before. However, as shown in f=figure 16 (A), on day 7, both groups had the same degree of infection, 50 °~ of the eyes are infected. However, beginning on day 10, a significant difference of the infection is seen between the two groups. For the group im-munized with monoclonal GLXA Ab2 IgG, on day 14, two out of eight eyes were positive, on day 22, one out of eight. No eye was positive on day 28, showing a Gear regression of the infection. In contrast, mice immunized with normal mouse IgG, on day 14, six out of six eyes were positive and continued to be positive until day 42. The number of infected eyes began to fall by day 28 seen in this group is believed to be a natural recovery pn~ss. In a final experiment, the mice with completely cleared infection from the above experiment were rechallenged with EBs in order to evaluate whether the immunity was associated with memory. A
signficant factor in terms of protecctieon is the ability of the immunized mice to clear the organisms from their eyes much earlier than the non-immunized ones. This is clearly shown to be the case with mice immunized with monoclonal GLXA Ab2 (Figure 16 (B)). This shows that monoclonal GL.X~4 Ab2 not only is able to evoke a *Trade-mark R'O 96/29604 PCT/LTS96/02617 protective immune response but also a memory immune response.
This example illustrates that an anti-idiotypic antibody which mimics GLXA, protects mice as an animal model from chlamydial ocular infection. The mono-y clonal antibody mAb~ (89MS30) which was used to produce anti-idiotypic an-tibodies was produced by immunization with whole EBs and screened for its reaction to a genus specfic antigen. It has been used to identify GLXA and demonstrated specific binding to the polysaccharide portion of GLXA. This antibody was also found cross-reactive to cLPS.
First GLXA and cLPS are distinctly different genus specific antigens. GLXA
was found on RBs, EBs, inclusion membranes, host cell membranes and shed into the inclusion space, cytoplasm of the infected cells and into the surroundings. It was obtained from the supernatant of, infected cell culture. Whereas cLPS was found both on EBs and RBs (mainly RBs). They are not secreted or shed from infected cells, but loosely bound to the RBs. Structurally, they have different polysaccharide moieties. GLXA has a unique sugar residue: gulose or gulose derivatives, mannose and galactose, probably arranged in repeating units of guluoronic and mannuronic acids. Only two fatty acids were found associated with the antigen compared to at least 12 in cLPS. Whereas cLPS has typical linear 2-keto-3-dexyoctonoic acid (KDO) trisaccharide (common core) and polysaccharides like glucosamiane and heptose. Serologically, monoclonal GLXA-Ab, specifically bind to gulose and mannose repeating block. Whereas, cLPS genus specific epitope is on KDO, the specific determinant is the 2-8 linkage. Obviously, it is very unlikely that GLXA and cLPS share the same epitope. It is known that antibodies, whether poly-or monoclonal, antibodies produced either by whole EBs or by purified cLPS which are specific to cLPS have no neutralizing or protective functions. From the composition analysis, it is suggested that gulose together with mannose and galactose form the specific epitope of GLXA. Whereas, cLPS, in addition to KDO trisaccharide as an epitope, has other epitopes in KDO region and also other saccharide portions. These later structures have shown a broad cross-WO 96/29604 PCT/US96l02617 reaction with LPS from other gram negative bacteria. Since the protective epitope of GLXA consists of an array of sugar residue, it is more reasonable to believe that some of which cLPS is partially shared with GLXA.
There are some other possibilities about this cross-reaction. For example, (1) GLXA and cLPS do not share any primary similarity, but structurally form similar binding motif; (2) although monoclonal GLXA Ab, binds to cLPS, GLXA .
and cLPS do not have the similarity in antibody binding site. The monoclonal antibody can be multispecific, that is, it recognizes a quite different epitope.
From the discussion above, it is believed that monoclonal GLXA-Ab, is specific to GLXA epitope, the possibility that GLXA and cLPS share same sugar residues or merely structure similarity may explain the cross-reactivity.
Identification of Receptor on Host Cells by Monoclonal GLXA-Ab 2 IgG
FACS analysis of the specific binding of monoclonal GLXA-Abz to HECEC cells Human endometria! gland epithelial cells (HECEC) were grown in a 75 mm2 flask at 37° C with 5% C02. When confluent, cells were scraped off the flask using a cell scraper (Baxter, 1L) and centrifuged 200 x g for 5 minutes. The cells were rinsed once with 20% FBS in Hanks buffer (Whittker, MD) and passed through a 19 G syringe needle four times to obtain single cells. Serial dilutions of biotin labeled monoclonal GLXA-Ab2 or biotin labeled normal mouse igG in Hanks buffer, (100 ul) were added to each vial which contained approximately 1.5 x 106 HECEC
cells and incubated otl ice for 30 minutes. Each vial was rinsed twice with 0.02%
azide in Hanks buffer. Later, 100 ul of FITC conjugated streptavidin was added and incubated for 30 minutes on ice. After washing twice, the cells were kept in 400 ul of sheath buffer on ice. Cells plus FITC conjugated streptavidin and cells alone were used as background control. Single color flow cytometry was perform-ed immediately by FACS scan (Becton Dickinson).

Anti-idiotypic antibodies, GLXA-Ab3 and monoclonal GLXA Ab2 Monoclonal GLXA Ab, was injected into guinea pigs subcutaneously in the absence of conjugate or Freund's adjuvant. All four immunized guinea pigs developed high titered anti-idiotypic antibodies specific to monoclonal Abp, which were found as early as 3 weeks after the first immunization. The titer was ap-proximately 1:5000 by ELISA. The production of the anti-idiotypic antisera contain a relatively high concentration of GLXA Ab2 which is specific to the hypervariable region of monoclonal GLXA-Ab,. This was shown after two absorptions by normal mouse IgG. When the IgG-1 isotype from guinea pig anti-idiotypic antibodies was used as an immunogen in three rabbits, the titer of anti-anti-idiotypic antibody was more than 1:20,000 two months after immunization. This demonstrates that immunoglobulin itself is a very potent immunogen. This is true not only for interspecies immunization, but also syngeneic immunization. Wth monoclonal anti-idiotypic antibody monoclonal GLXA-Ab2, the immunization was carried out in syngeneic mice without KLH-conjugation or Freund's adjuvant. The mice de-veloped high titered GLXA-Ab3 in a short time after immunization (9 days). The protocol used in this study is different from most methods which use either a conjugate or Freund's adjuvant for a higher immunogenicity.
A successful vaccine not only requires that it be a good immunogen but that it is long lasting (preferably for the lifetime off the host). The immunity produced by idiotype is long lived. The ability to inhibit the binding of monclonal GLXA Ab, to GLXA by guinea pig GLXA Ab2 from three immunized guinea pigs have been monitored for as long as 77 weeks. With only three boosts, the inhibition one year post immunization is almost equal to antisera collected in the early stages after the immunization. This indicates that the immunity elicited by the idiotypic antibody monoclonal GLXA-Ab, has a long term memory. Since the half life of an antibody molecule or the majority of antibody-producing cells is about a few weeks, the boosting interval (six months) is far beyond the life span of the B cells and the immunoglobulins. It is the constant stimulation within the idiotypic network that keeps this anti-idiotypic antibody at a certain level. The change of idiotypic specificity during this period has not been seen in this case.
An internal image of chlamydial GLXA, isotypic difference In this study, guinea pig GLXA-Ab2 IgG-1 and BgG-2 were separated. The regulatory function of these two isotypes to the idiotype was not evaluated.
However, the difference between IgG-1 and IgG-2 subclasses have been found in inhibition of the binding of monoclonal GLXA-Ab, to GLXA. With a novel system, chemiluminometric immune-assay, the incubation and the final detection were all carried out in solution rather than solid phase as in ELISA, thus greatly lessening the possibility of the inhibition by hindrance. The results have shown that GLXA-Ab2 IgG-1 inhibited 100% of the binding whereas IgG2 50% at the same con-centration. This suggested that GLXA-Ab2 IgG-1 has a high affinity in binding to the idiotype or being more like the antigen, GtXA. This demonstrates an isotypic difference in their binding ability to the idiotype which reflects a difference in their respective active sites. IgG-1 has a different idiotype binding ability from IgG1.
There are a number of examples of dominant idiotypes, for example, A5A
idiotope of anti-strep-A carbohydrate antibodies or the T15 idiotope of phosphoryl choline antibodies. It is not clear if there is any isotype preference of anti-idiotypic antibody in different systems. This finding suggests that a certain isotype of GLXA Ab2 is the internal image while others are not.
Monoclonal GLXA-Ab2 as an immunogen of chlamydial GLXA
The purpose of making monoclonal anti-idiotypic antibodies is to: (1) have a constant source of anti-idiotypic antibody for vaccine study; (2) identify a possible receptor for GLXA on host cells; and (3) further characterize the epitope on GLxA.
This enables an understanding of biological functions of GLXA in terms of epitope density, its role in mechanism of infection and the protective function against chla-mydial infection in vivo. The production of monoclonal anti-idiotypic antibodies was carried out in the syngeneic BALB/cBYJ mice. In the first fusion, one stable, highly inhibitory clone (91 MS441 ) from 283 clones screened was selected. In the second fusion, another clone (99 MS442) was selected though it is not as inhibitory as 91 MS441 clone in chemiluminometric immunoassay. The monoclonal GLXA
Ab2 produced by this clone (91MS441) has been shown to be the internal image of the chlamydial antigen, GLXA.
It is interesting to note that the inhibitory ability of mouse GLXA-Ab3 slightly but obviously decreases over time. The dosage of the anti-idiotype has been a factor in either enhancing the idiotype or suppressing the idiotype. This inhibition results by GLXA-Ab3 has shown that after administration of monoclonal GLXA-Ab2 IgG twice, the inhibition is higher than the sera obtained after administration three times. This indicated 50 ug is either too much for one dose or too much for repeated administrations. On the other hand, it shows that a low amount is enough for protective immunity. The reason for choosing normal mouse IgG as a negative control in the immunization rather than a non-relative clone is that it would prevent any possible bias from a specific clone.
Monoclonal G~XA-Ab, and GLXA-Ab3 bear the same antigen binding structure.
GLXA Ab3 from immunized rabbits and mice recognized affinity purified GLXA by immune-dot blot assay, though there is no previous exposure to G(xA or infection. The binding of monoclonal GLXA Ab, to GLXA is inhibited as the concentration of GLXA-Ab3 increases. This indicates that the anti-anti-idiotype has equivalent antigen reactivity as idiotype, that is they recognize the same epitope.
The same antigen reactivity of monoclonal GLJCA Ab, and GLXA-Ab3 from rabbits to GIJCA was further proved in the immune-fluorescent staining of the inclusions in infected McCoy cell culture. The experiment suggested the structural similarity of antibodies. Using monoclonal GLXA-Ab2 which mimic GLXA to identify its role R'O 96/29604 PCT/US96/02617 would be valuable in understanding the mechanism of anti-idiotype protection.
The experiment was carried out with human epidermoid carcinoma cells (A431 ) as well as human endometrial gland epithelial cells (HEGEC). Those cell lines were used because of their human origin. A preliminary binding experiment was performed by direct antibody staining detected with FACScan (Becton Dickinson, N.J.) flow cytometer. Since the separation of these epithelial cells into a single cell suspen-sion is very difficult without using enzyme or harsh separation, especially HEGEC
cells, the cell population consists of singlets, doublets and multiplets.
Single cell population was gated right above the cell debris. Since the control, cells stained with normal mouse IgG was at exactly the same gate, it is believed that the two groups are comparable. In addition, the binding is direct, monoclonal GLXA-Ab2 or normal mouse IgG .was directly biotin labeled. The intensity of monoclonal GLXA-Ab2 bound increases with the concentration specifically to the host cells (HEGEC).
While normal mouse IgG has no such binding even at the highest concentration.
tf this finding can be repeated and proved to be valid, GLXA is an adhesion or a ligand which binds to HEGEC cells. There are some reasons to believe that GLXA
is an adhesion or a ligand. First, as mentioned above, GLXA Ab3 neutralization occurs at the very early stage. This is proved by finding apparently no significant chlamydial specific ribosomal RNA in conjunctiva samples taken from primates inoculated with GLXA-Ab 3 treated EBs. This suggested that GLXA-Ab 3 blocked EBs from getting into the host. Second, Gt.XA was found to enhance the infection by approximately three fold when McCoy cells were pre-incubated with GLXA. It is only if GLXA as an adhesion or ligand which facilitate the attachment of EBs to host cells that this result can occur. Actually, EBs may well use this mechanism to infect host cells because GL.XA are secreted from infected cells.
A possible mechanism of the role of GLXA may be the following: EBs attach.
to the host cells either by GLXA on EBs or by free GLXA which were secreted by the infected cells into the surroundings. This makes it much easier and efficient for GIxA to absorb to surrounding cells. Ebs can then attach to the host cells either by GLXA on EBs, thus binding to the host cells. This mechanism seems much more efficient than vne to one attachment.
Neutralization of chlamydial infection by GLXA-Ab3 The preliminary .neutralization test in vitro has shown that more chlamydial inclusions were found with GLXA-Ab, treated than rabbit Ab3 treated C.
trachoma-tis serovar B EBs. This showed that GLXA-Ab3 neutralized the infection, whereas monoclonal GLXA-Ab, did not. GLXA-Ab3 neutralized the infection in cell culture whereas monoclonal GLXA-Ab, did not. This in vitro result was repeated in vivo in two later experiments with the primate infection model. It was confirmed that GLXA-Ab3 effectively neutralized chlamydial infection both in vitro and in vivo.
The understanding of the mechanism of this neutralization comes from the chlamydia specific RNA hybridization experiment. The primates were ocularly inoculated with GLXA Ab3 or normal rabbit 1gG treated EBs. Chlamydial RNA was detected from the conjunctiva) swabs taken from primates on different days prior and post inoculation. The RNA hybridization assay used in this study is an extremely sensitive way to detect chlamydial infection in samples which are unequivocally negative by either cell culture of DFA or both. The substantially low RNA found in Ab3 treated primates provides the evidence that the neutralization occurs at very early stage of the infection, before the internalization of the or-ganisms. This suggests that GLXA may be an adhesion or ligand functioning at the stage of attachment.
The role of humoral immunity in protection against chlamydial infection has long been discrepant. However, it has been shown both in vitro and in vivo that humoral immunity may play some role in preventing chlamydial infection.
Protection of Mice from chlamydial infection by immunization with monoclonal GLXA-Ab2 The chlamydial ocular infection model in BALB/cByJ mouse was employed in a vaccine study with monoclonal anti-idiotypic antibody monoclonal GIXA-IgG.
It is model for C. trachomatous serovars which only infect humans. In the im-munization experiments, monoclonal (GLXA-Ab2) IgG (50 ug/mouse) was used to immunize 6 to 20 mice in each group subcutaneously either in the presence of adjuvant or with no adjuvant. Mice immunized with monoclonal GLXA-Ab2 mount a distinctive GLXA-Ab3 titer detectable one week after a single immunization.
The system used in this study is syngeneic: monoclonal GLXA-Ab,, monoclonal GLXA
Ab2 or GLXA-Ab3 are all produced in the same strain of mice. They bear the same immunoglobulins genetically. The only "foreign structure" is the specific binding site of each type antibody (monoclonal GLXA-Ab, or monoclonal GLXA-Ab2).
Normal mouse IgG from the same strain was used as a negative control. Con-sistently, mice immunized with monoclonal GLXA-Abz developed a significantly high GLXA-Ab3 titer against purified GLXA compared to the control group. The average titer was as high as 1:3200 comparing with 1:200 in the mice immunized with normal mouse IgG. This clearly demonstrates that the production of GLXA-Ab3 antibody in synergenic mice is elided by the hypervariable region, the struc-ture which mimics the GtXA. In addition, the GLXA-Ab3 from these mice inhibited the binding of monoclonal GLXA-Ab, to GLXA as efficiently as unlabeled mono-clonal GLXA-Ab,. These experiments shows that monoclonal GLXA-Ab2 mimics one single epitope of GLXA.
The protection of mice from ocular infection by C. trachomatous was consistently demonstrated in four individual experiments in vivo. The mice immunized with monoclonal GLXA Ab2 or normal mouse IgG (three times on a weekly basis) were infected in the eyes by inoculation of EBs (5000 IFU/eye).
The conjunctival swabs were taken on different days before and after the infection.
Inclusions were detected by cell culture. The eyes of the mice immunized with monoclonal GLXA-Ab2 IgG have significantly short recovery (9 days after ocular inoculation comparing to 28 days of the control immunized with normal mouse IgG). The GLXA-Ab3 titer is well correlated with cell culture results. This demon-strates that monoclonal GLXA-Ab2 which mimics a single GLXA epitope, is an effective immunogen, and evokes a strong protective immune response against chlamydial infection. This shows that a single protective epitope resides on chlamydial GLXA.
Prospective of the mechanism of the neutralization and protection This example is the first demonstration that a non-neutralizing monoclonal GLXA Ab, can produce a neutralizing GLXA-Ab3 in vivo through an anti-idiotypic antibody (GLXA-Ab2). The central issue is that monoclonal GLXA Ab, produced by immunization with chlamydial EBs does not neutralize or protect primates from reinfection whereas GLXA Ab3 produced by guinea pig GLXA-Ab2 neutralized the infection and immunization with monoclonal GLXA-Ab2 protects mice from reinfec-tion.
Assay results in Examples 2-5 for the presence of GLXA in in vitro and in vitro (including cellular and non-cellular material) samples are as follows:
GLXA has been found to be present in Chlamydia EB suspensions prepared from in vitro cell culture when assayed in Examples 2, 3, 4 and 5.
GLXA has been found to be present in Chlamydia infected in vitro cell culture .supernatants when assayed in Examples 2 and 4.
GLXA has been found to be present in cervical swab specimens from cell culture confirmed Chlamydia infected females when assayed in Examples 3,4 and 5.
GLXA has been found to be present in vaginal swab specimens from cell culture confirmed Chlamydia infected females when assayed in Example 5.
GLXA has been found to be present in urine specimens from cell culture confirmed Chlamydia infected females when assayed in Examples 4 and 5.
Example 2 A sandwich ELISA assay.
Polystyrene microliter plate wells are coated with rabbit polyclonal antisera containing anti-GLXA antibodies (GLXA Ab,).
Monoclonal anti-GLXA antibody (GLXA-Ab,) is conjugated to horseradish peroxidase (HRP).
Assay Protocol: . -1 ) Pipet 100 ul of sample per well 2) Pipet 100 ul of assay buffer per well. ' 3) Incubate for one hour @ 37° C. , 4) Wash the wells 3X with PBS/tween, blot dry.
5) Pipet 200 ul per well monoclonal anti-GLXA: HRP conjugate.
6) Incubate for one hour @ 37° C.
7) Wash the wells 2X with PBS/tween then 2X with PBS, blot dry.
8) Pipet 200 ul per well substrate/chromogen solution.
9) Incubate for 30 minutes @ room temperature.
10) Stop the reaction by pipetting 100 ul per well 1 N H2S04.
11 ) Read the absorbance of each well in a spectrophotometer.
Examale 3 An amplified sandwich ELISA assay.
Polystyrene microliter plate wells are coated with monoclonal anti-GLXA
antibody (GLXA-Ab,). Monoclonal anti-GLXA antibody if biotinylated. Monoclonal anti-Biotin antibody is conjugated to horseradish peroxidase (HRP).
Assay Protocol:
1 ) Pipet 140 ul of assay buffer per well , 2) Pipet 10 ul of sample per well.
3) Incubate for 30 minutes @ room temperature.
4) Wash the wells 3X with PBSfiween, blot dry.
5) Pipet 150 ut per wel! biotinylated anti-GLXA antibody.
6) Incubate for 30 minutes @ room temperature.
7) Wash the wells 3X with PBS/finreen, blot dry.
8) Pipet 150 ul per well anti-biotin: HRP conjugate.

WO 96/29604 PC~YUS96/0261'7 9) Incubate for 30 minutes @ room temperature.
10) Wash the wells 5X with PBS/tween, blot dry.
11) Pipet 150 ul per well substrate/chromogen solution.
12) Incubate for 6 minutes @ room temperature.
13) Stop the reaction by pipetting 100 ul per well 1 N H2S04.
14) Read the absorbance of each well in a spectrophotometer.
For the sandwich ELISA assays the final absorbance in each well is directly proportional to the amount of GLXA in the sample. Any absorbance greater than 2X the absorbance of the negative control is indicative of the presence of GLXA in the sample.
Example 4 A competing ELISA assay.
Polystyrene microliter plate are coated with monoclonal anti-GLXA antibody (GLXA-Ab,). Monoclonal anti-idiotypic antibody GLXA-Ab2) is conjugated to horse-radish peroxidase (HRP).
Assay Protocol:
1 ) Pipet 200 ul of sample per well 2) Incubate for one hour @ 37° C.
3) Pipet 100 ul per well GLXA-Ab2 :HRP per well.
4) Incubate for 30 minutes @ room temperature.
5) Wash the wells 4X with PBS/tween, blot dry.
6) Pipet 200 ul of substrate/chromogen per well.
7) Incubate for 20 minutes @ room temperature.
8) Stop the reaction by pipetting 100 ul per well 1 N H2S0,,.
9) Read the absorbance of each well in a spectrophotometer.
Example 5 . An amplified competitive ELISA assay. Polystyrene microtiter plate wells are coated with monoclonal anti-idiotypic antibody (GLXA-Ab2). Monoclonal anti-GLXA (GLXA-Ab,) antibody is biotinylated. Monoclonal anti-biotin is conjugated to horseradish peroxidase (HRP).
1 ) Pipet 100 ul ofi assay buffer per well 2) Pipet 30 ul of sample per well 3) Pipet 20 ul of biotinylated GLXA Ab, per well.
4) Incubate for 45 minutes @ room temperature.
5) Wash the wells 3X with PBS/tween, blot dry.
6) Pipet 150 ul of anti-biotin: HRP conjugate per well.
7) Incubate for 45 minutes @ room temperature.
8) Wash the wells 5X with PBS/tween, blot dry.
9) Pipet 150 ul per well substrate/chromogen solution.
10) Incubate for 5 minutes @ room temperature.
11 ) Stop the reaction by pipetting 100 ul per well 1 N H2S04.
12) Read the absorbance of each well in a spectrophotometer.
For the competitive ELISA assays the final absorbance in each well is inversely proportional to the amount of GLXA in the sample. The % inhibition is calculated by the formula:
inhibition = ffAbs nea control) - (Abs. sample)1 X 100%
Abs. neg. control Any inhibition greater than 20% is indicative of the presence of GLXA in the sample.
Assay results for the presence of GLXA in in vitro and in vivo (including cellular and non-cellular material) samples are as follows:
GLXA has been found to be present in Chlamydia EB suspensions prepared from in vitro cell culture when assayed in the above example assays #s 2, 3, 4 and 5.
GLXA has been found to be present in Chlamydia infected in vitro cell , culture supernatants when assayed in the above example assays #s 2 and 4.
GLXA has been found to be present in cervical swab specimens from cell culture confirmed Chlamydia infected females when assayed in the above example assays #s 3, 4 and 5.
GLXA has been found to be present in vaginal swab specimens from cell culture confirmed Chlamydia infected females when assayed in the above example assays # 5.
GLXA has been found to be present in urine specimens from cell culture confirmed Chlamydia infected females when assayed in the above example assays #s 4 and 5.

Claims (10)

CLAIMS:
1. A method for immunochemically diagnosing Chlamydia in a mammal which method comprises:
contacting an extracellular biological fluid from said mammal with antibody specific for a genus-specific Chlamydial glycolipid exoantigen; measuring any specific binding immunocomplexes formed between the antibody and any Chlamydial glycolipid exoantigen present in the fluid; and comparing the amount of the immunocomplexes formed in the fluid with the amount of immunocomplexes formed by a control fluid from a mammal free of Chlamydia infection, wherein a greater amount of immunocomplexes in the fluid than that found in the control fluid indicates the presence of Chlamydia infection in the mammal.
2. The method according to claim 1 which method comprises determining the amount of glycolipid exoantigen in the extracellular biological fluid via a competitive immunoassay utilizing an anti-idiotypic antibody that contains an internal image of the specific epitope of Chlamydial glycolipid exoantigen.
3. The method according to claim 1 wherein the immunocomplexes are measured by an immunochemical assay selected from the group consisting of radioimmunoassay, enzyme-linked immunosorbent assay, fluorescent assay, chemiluminescent assay, bioluminescent assay, competitive immunoassay, membrane-based immunoassay, precipitation, agglutination and antigen capture.
4. The method according to claim 1 wherein the antibody specific for Chlamydial glycolipid exoantigen is monoclonal.
5. The method according to claim 1 wherein the antibody specific for Chlamydial glycolipid exoantigen is polyclonal.
6. The method according to claim 2 wherein the anti-idiotype antibody that contains the internal image of the specific epitope of Chlamydial glycolipid exoantigen is monoclonal.
7. The method according to claim 2 wherein the anti-idiotype antibody that contains the internal image of the specific epitope of Chlamydial glycolipid exoantigen is polyclonal.
8. The method according to claim 1 wherein the antibody specific for Chlamydial glycolipid exoantigen is an anti-anti-idiotypic antibody.
9. The method according to claim 8 wherein the anti-anti-idiotypic antibody is polyclonal.
10. The method according to claim 8 wherein the anti-anti-idiotypic antibody is monoclonal.
CA002215528A 1995-03-17 1996-02-28 Method for diagnosing a patient for chlamydia Expired - Fee Related CA2215528C (en)

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US08/406,113 US5716793A (en) 1993-03-19 1995-03-17 Method for diagnosing a patient for chlamydia
US08/406,113 1995-03-17
PCT/US1996/002617 WO1996029604A1 (en) 1995-03-17 1996-02-28 Method for diagnosing a patient for chlamydia

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