WO1999012038A1 - Detection of measles virus-specific antibodies - Google Patents
Detection of measles virus-specific antibodies Download PDFInfo
- Publication number
- WO1999012038A1 WO1999012038A1 PCT/EP1998/005546 EP9805546W WO9912038A1 WO 1999012038 A1 WO1999012038 A1 WO 1999012038A1 EP 9805546 W EP9805546 W EP 9805546W WO 9912038 A1 WO9912038 A1 WO 9912038A1
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- WIPO (PCT)
- Prior art keywords
- elisa
- measles
- sera
- measles virus
- virus
- Prior art date
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Definitions
- the present invention relates to a method for the identification of measles virus specific antibody in a sample, comprising contacting a sample suspected of containing measles virus specific antibody with a measles virus specific glycoprotein recombinantly produces in mammalian cells using a high expression system; and detecting the presence or absence of said measles virus specific antibody in said sample.
- the expression system is based on a togavirus expression system, more preferred on an alphavirus expression system, and most preferred on a Semiiki Forest virus expression system.
- the present invention relates to a kit comprising said recombinantly produced glycoproteins.
- the method of the present invention allows an easy and reliable assay of the immune status of the human with respect to the present or past infection with measles virus.
- Measles is a major word-wide health problem. In developing countries 60 million cases are reported each year, with a mortality of approximately 1 million children. In the industrialised countries eradication of measles remains elusive and despite vaccination programmes out-breaks continue to occur. Considering the failure to control measles in the developed countries and the continuing high measles related mortality in the developing countries there is a continuing need for improved methods for monitoring immunity and for diagnosis. This need becomes even more urgent, since rare and isolated cases tend to become more difficult to diagnose clinically. Also, diseases with similar skin involvement such as allergies are becoming more frequent while measles tends to become less frequent. With the frequency of measles patients decreasing, medical personnel tends to loose the experience for diagnosing this disease.
- the measles eradication programme of the Word Health Organisation requires an intensive surveillance of measles immunity world-wide. Therefore, surveillance of measles epidemiology and immunity will rely increasingly on serological parameters.
- Measles immunity consists of cellular and humoral effector mechanisms. Cellular immunity is normally not measured directly and the relevance of serum immunoglubulins to susceptibility and immunity is an open issue. Different serological assays measure different subsets of antibodies, but it is not clear which subset reflects the overall immune status. For an antigenic component of the measles virus to be useful for monitoring measles or measles immunity it is critical that the immunoglobulins generated against the measles virus component accurately reflect the measles immune status.
- the antigenicity of the antigen used in the immune assay for detecting said immunoglobulins must sufficiently resemble the virus and unspecific binding to the antigen preparation must be low. After contact with measles antibodies are generated against different antigenic components. These include the nucleoprotein and surface glycoproteins.
- Detection of specific IgM by EIA can be performed in different ways.
- the serum may be pretreated to remove interfering IgG antibodies.
- serum IgM is immobilised to the solid support using an anti-human IgM antibody (Erdman et al. 1991 J. Clin. Microbiol. 29: 1466-1471 ).
- Diagnosis of measles may be confirmed by virus isolation, by the demonstration of a significant increase in specific immunoglobulin G (IgG) titers, or by the detection of anti-measles virus (MV) IgM antibodies using radioimmunoassays (Arstila et al. 1977 J. Gen. Virol. 34:167-176; Jankowski et al. 1982 Acta Virol. 26:481-487; Vuorimaa et al. 1978 J. Virol. 2:271-278), enzyme-linked immunosorbent assays (ELISA) (Pedersen et al. 1982 Acta Path. Microbiol. Immunol. Scand. Sect. B.
- radioimmunoassays Asrstila et al. 1977 J. Gen. Virol. 34:167-176; Jankowski et al. 1982 Acta Virol. 26:481-487; Vuorimaa et al. 1978 J. Virol. 2:271-278
- IgM peaks on day 7 to 10 and wanes within weeks (Pederson et al. 1986 Vaccine 4:173-178). Since IgM is transient, the demonstration of specific IgM corresponds to a recent primary measles infection (Helfand et al. 1997 J. Infect. Dis. 175:195-199; Lievens and Brunell 1986 J. Clin. Microbiol. 24:391- 394). A single serum specimen collected at the appropriate time (Helfand et al.
- recombinant proteins of the measles virus produced by gene technology in heterologous host cells are an alternative to whole virus as antigen.
- Such a system provides a virtually unlimited supply of measles antigens suitable as antigen for detecting measles-specific antibodies.
- expressing proteins by recombinant means would also allow for lower batch to batch variation and greater ease in calibrating and quantifying assays.
- Mammalian expression systems may, however, also have some disadvantages: Usually the expression is to low to efficiently produce large amounts of the recombinant antigen; due to close contacts between humans and other mammals antibodies against mammalian tissues may cause elevated background levels against contaminating cell debris. In addition, complicated steps may be required to isolate the antigen with sufficient purity.
- the technical problem underlying the present invention therefore was to overcome the above recited problems and to provide a conveniently usable and reliable detection system for measles virus glycoprotein induced antibody formulation.
- the present invention relates to a method for the identification of measles virus specific antibody in a sample comprising (a) contacting a sample suspected of containing measles virus specific antibody with a measles virus specific glycoprotein recombinantly produces in mammalian cells using a high expression system; and (b) detecting the presence or absence of said measles virus specific antibody in said sample.
- identification as used in accordance with the present invention in its broadest aspect is intended to mean that it is determined whether such antibodies are at all present in said sample. Said term further comprises the quantitative and/or qualitative measurement of such antibodies such as the isotype determination.
- isotype determination also comprises isotype subclass determination.
- measles virus specific antibody in accordance with the present invention, is intended to mean any antibody that essentially only reacts with epitopes specific for a measles virus antigen. Accordingly, said antibody does not or does not significantly cross-react with any other antigen such as antigens of viruses other than measles viruses that belong to the family Paramyxoviridae.
- measles virus specific glycoprotein is intended to mean any full-length glycoprotein that corresponds to the naturally corresponding glycoproteins.
- said term comprises fragments and derivatives of said glycoproteins that retain the or at least part of the epitope specificity of said naturally occurring measles virus antigens.
- the antigens can be the native antigens or can be modified versions thereof.
- Well known techniques of molecular biology can be used to alter the amino acid sequence of a measles antigen to produce modified versions of the antigen that may be used in accordance with the invention. These techniques are useful to alter patterns of post-translational modification. For instance, changes in the amino acid sequence of a protein can alter its glycosylation or phosphorylation pattern. Such techniques are also useful to provide specific functional moieties that aid efficient expression or purification of recombinantly expressed proteins, inter alia.
- recombinantly produced comprises any production method that employs recombinant DNA technology. It will be readily evident for the person skilled in the art that "recombinant DNA technology” is not restricted to DNA only but comprises any recombinant nucleic acid technology like, e.g., also recombinant RNA technology.
- the present invention overcomes many of the disadvantages of the conventional methodology for detecting measles-specific antibodies by allowing one to readily make recombinant measles antigens that serve as sensitive detectors in enzyme immunosorbent assays ("EIAs”) and other immunoiogical assays.
- EIAs enzyme immunosorbent assays
- the method of the invention involves constructing a plasmid DNA, or the like, in which a DNA sequence that encodes a protein of antigenic potential which serves as template for in vitro synthesis of recombinant RNA which can be used both for direct transfection of appropriate host cells as well as production of recombinant virus that only expresses the heterologous portion of a recombinant protein.
- a DNA sequence that encodes a protein of antigenic potential which serves as template for in vitro synthesis of recombinant RNA which can be used both for direct transfection of appropriate host cells as well as production of recombinant virus that only expresses the heterologous portion of a recombinant protein.
- the recombinant RNA drives its own replication and capping and its own transcription of RNA molecules and leads to massive production of the antigen of interest while competing out the host protein synthesis. See, e.g., Liljestr ⁇ m and Garoff (1991 ) BioTechnology 9:1356-1361
- a variety of expression systems may be used to produce measles antigens in accordance with the invention.
- a variety of expression vectors suitable to producing proteins in systems including vaccinia virus (Wild et al. 1992, J. Gen. Virol. 73:359-367; Taylor et al. 1991 , J. Virol. 65:4263-4274; Drillien et al. 1988, Proc. Natl. Acad. Sci. U. S. A. 85:1252-1256), canarypox virus (Taylor et al. 1992, Virology 187:321-328), adenovirus (Alkhatib and Briedis, 1988, J. Virol.
- Antigens produced in accordance with the invention can be used in a variety of immunoiogical assays to detect anti-measles antibodies in an individual which was exposed to or infected by measles virus.
- antigens according to the invention can be used in place of natural virus in practically any immunoiogical assay for detection of measles- specific antibodies.
- the assays include direct and indirect assays, sandwich assays, solid phase assays such as, e.g., those using plates, beads, electronic sensory devices such as electronic sensory chips or any other solid support, and liquid phase assays, inter alia.
- Assays suitable for use in the invention include those that use primary and secondary antibodies, and those that use antibody binding reagents such as protein A.
- detection methods can be used in the invention, including colorimetric, fluorescent, phosphorescent, chemiluminescent, luminescent and radioactive, dye concentrating methods, and other detection methods.
- the present invention is further described by reference to the following, illustrative examples. In these examples, a variety of antibodies were used. The antibodies were produced according to conventional methods and could have been replaced by similar antibodies.
- said measles virus specific glycoprotein is the hemagglutinin (H) or the membrane fusion protein. Also comprised by this embodiment is the consecutive or simultaneous use of both glycoproteins for the identification of measles virus specific antibody.
- the measles virus genome is a negative single-stranded RNA encoding for a small number of viral proteins.
- the immune response antibodies are generated against the different proteins including the hemagglutinin protein encoded by the H gene, the fusion protein encoded by the F gene and the nucleoprotein encoded by the N gene (Giraudon and Wild 1985 Virology 144:46-58. Malvoisin and Wild 1990 J. Virol. 64:5160-4. Graves et al. 1984 J. Virol. 49:409. Norrby et al. 1981 Infect Immun. 34:718).
- Antibodies can prevent measles virus proliferation in vitro as measured by neutralisation assay.
- the hemagglutinin protein and the fusion protein combine several properties relevant to this invention: they are (1 ) membrane proteins, (2) glycosylated, (3) target proteins of virus eliminating antibodies; (4) potentialy more stable than the whole virus; (5) further more immunoglobulins against these proteins occur during measles infection; (6) antibodies against these proteins persist life long in an individual having been exposed to measles virus either during measles or after vaccination.
- the antibody response against the hemagglutinin reflects the antibody response against the whole measles virus.
- Nucleoprotein specific antibodies may appear somewhat earlier during measles infection and are thought to be the most abundant antibodies early after onset of rash (Graves et al. 1984 J. Virol. 49:409-412; Norrby and Gollmar 1972 Infection and Immunity 6:240-247; Pedersen et al. 1982 Acta Path. Microbiol. Immunol. Scand. Sect. B. 90:153-160), but this protein shows considerable sequence variability (Rima et al. 1995 Vet. Microbiol. 44:127-134). In contrast, lower levels of H-specific antibodies were detected by immunoprecipitation (Graves et al. 1984 J. Virol.
- said high expression system is based on a togavirus expression system.
- said togavirus is an alphavirus.
- said alphavirus is Semliki Forest virus or Sindbis virus.
- the high yield expression systems of the invention based, e.g., on the Semliki Forest Virus system (Liijestr ⁇ m, P. and H. Garoff. 1991 BioTechnology 9:1356-1361 ; Berglund et al. 1993, BioTechnology 11 :916-920) can be used to express large quantities of foreign proteins and, in accordance with this invention, can provide the necessary processing.
- RNA produced in vitro or belonging to a recombinant SFV particle encoding the antigen
- recombinant RNA comprises the SFV replicase-encoding gene nsP1-P4 followed by a promoter for subgenomic transcription of the antigen RNA sequence.
- This recombinant RNA allows the expression of the antigen in a wide range of mammalian cells after direct transfection of cells with (a) the recombinant SFV RNA produced in vitro or (b) a DNA vector which directs in vivo the synthesis of the recombinant SFV RNA transcripts or after infection of cells with a recombinant RNA packaged in vivo into SFV particles using cotransfection with packaging-deficient helper RNA molecule.
- the recombinant RNA drives its own replication and capping and its own transcription of RNA molecules and leads to massive production of the antigen of interest while competing out the host protein synthesis.
- the Semliki Forest Virus replicon consisting of a self- replicating and self-transcribing molecule using host cell transcriptionai machinery system is most preferred because of the high yield of expression.
- the SFV expression system is preferably used in combination with hamster kidney cell lines such as BHK-21 (see appended examples or e.g. ATCC CCL 10, ATCC CRL 8544).
- Semliki Forest virus expression system comprises plasmid pSFVI-MVH, the construction of which is shown in Example 1.
- said sample is derived from a body fluid.
- said body fluid is serum, plasma, saliva or cerebrospinal fluid.
- said body fluid is obtained from a patient infected with measles virus, a convalescent having recovered from measles virus infections, a subject immunized with a measles vaccine or a sero-negative individual.
- Measles virus-specific antibodies are mainly found in the blood (i.e. the plasma or the serum) and to a lesser extent in mucosal fluids such as saliva.
- the presence of MV-neutralizing and hemagglutination inhibiting antibodies is thought to reflect the immune status of the individual. In particular, these permit to distinguish between individuals with and without immunity against measles.
- glycoprotein specific antibodies are a better measure of measles immunity than whole measles virus specific antibodies, since specificity, accuracy, positive as well as negative predictive value were better. Both assays did not significantly differ by the numbers of false negative sera. In contrast, the whole virus based ELISA had significantly more false positive sera than the H-ELISA.
- Measurements of specific measles-lgG is, most importantly, supposed to predict susceptibility to measles infection. In any given cohort, only few individuals will be seronegative for measles. Among these, false positive donors are at risk of disease and can support viral circulation. Identification of such false positive sera would require retesting most sera by using a different assay. On the other hand, individuals tested false negative have no enhanced risk and are epidemiologically irrelevant. Also, rare false negative sera could in principle be retested (with another assay) or such individuals could simply be (re-)vaccinated. For these reasons, false negative results can be better tolerated than false positive results, which were absent in the assay performed in accordance with the invention.
- the H-ELISA in contrast to the MV-ELISA, detects no false positive sera, indicating that the recombinant assay may be more efficient in detecting vaccine failure than conventional assays, which is the main purpose of a IgG detection assay.
- IgG detection assay After vaccination only few individuals will not seroconvert; they will be at risk of disease and support viral transmission. If they are tested false positive, they will not be detected. In contrast, a false negative result represents no risk for the individual concerned nor for his contacts. The few persons with false negative sera could simply be revaccinated together with true negative individuals.
- H-specific antibodies are functionally the most important antibodies, their contribution to protection in the two groups is probably the same.
- MV-de ved antigens are necessary, which can be incorporated into a simplified field test.
- said antibody is an IgG, IgA or an IgM antibody.
- Specific IgM develop only after a first measles virus infection or vaccination. Therefore the detection of specific IgM antibody can be used to diagnose a fresh measies infection, while the detection of IgG indicates that immunity against measles has developed.
- Specific IgA develops in the blood and on mucosal surfaces such in saliva. Thus, the detection of IgA, IgG and IgM permits distinguishing between fresh measles infection and immunity.
- said glycoprotein is affixed to a solid support.
- said solid support is a well of a microtitre plate, a bead, an electronic sensory device or any support compatible with a rapid test format.
- said solid support is comprised in a crude cell extract.
- expression systems and preferably the SFV expression system which is preferably used in conjunction with BHK 21 cells do not contain components which interfere with the detection of antibodies in the method of the invention in the sense that they would artificially enhance signals: as a result the number of false positive sera remains very low. Further purification of the antigen, although not necessary would only improve the characteristics of the assay.
- the cell extract may be at least partially purified and an extract comprising the measles glycoprotein(s) be used in the method of the invention.
- said detection is obtained without the computation of background values.
- Inexpensive and simple tests which could be used under field conditions, as an alternative to whole virus-based ELISA would represent an important step towards measles control.
- ELISAs based on recombinant proteins would potentially benefit from enhanced stability of the antigen which at the same time provide expressive and reliable data and which can be incorporated into a simplified field test.
- Such a test requires antigen preparations which give a constant background so that a background subtraction is not necessary, and the result is obtained as a single value read-out.
- the present invention demonstrates that the combination of the expression system with the antigen and the antigen preparation results in an assay with a stable unspecific binding where background subtraction is not necessary. The short time required for the developement represents another considerable advantage. Even when using 30 min raw data no false positive serum was found. Although under these conditions the number of false negative sera increases in comparison to net data, it still compares favorably with the MV-ELISA.
- said identification comprises the identification of specific measles strains.
- Differences in strain characteristics may be due to the local origin of said virus. Since it is well known that measles virus strains such as from different origins of the world have, as a rule, at least slightly different immunoiogical characteristics such as at least slightly different epitopes, the panel of antibodies generated thereto varies with virus strains. Accordingly, antigens, such as H antigens recombinantly produced from different MV strains will yield different read-out intensities when tested in e.g. conventional immunoassays, such as ELISAs with one and the same serum from e.g. a sero-positive individual. The interpretation of the data obtained with such a test system will allow the person skilled in the art to draw conclusions with respect to the nature and/or origin of the virus strain.
- the invention also relates to a kit comprising (a) recombinantly produced glycoproteins as identified in any of the preceeding methods either in solution or immobilized on a solid support; and
- Such reagents may be, for example, antibodies specific for human antibodies which are coupled to a detectable marker.
- the kit of the invention may contain the H protein of one or several vaccine strains and/or of one or several wild-type strains.
- the combination of H protein molecules derived from different viruses will serve to identify different measles virus strains which have induced immunity in a given individual.
- the kit of the invention may be used for any of the purposes described herein above.
- Figure 1 is a schematic diagram showing the strategy for the construction of recombinant plasmids used in the reconstitution of the full-length cDNA of the recombinant H protein and its transfer to the expression vector pSFV-1. Restriction endonuclease digests were performed as indicated by hatched and strippelt areas representing coding regions of the measles H protein and the vectors or plasmids used.
- Figure 2 shows the detection of recombinant H protein (panel A) on transfected BHK-21 cells (BHK-H) with an anti-MV mAb (BH47; Fournier et al. 1997. J Gen. Virol. In press) by flow cytometry.
- An MV fusion protein-specific mAb (A352; anti MV-F) served as an irrelevant control antibody; beta-galactosidase transfected BHK-21 cells (BHK-gal, panel B) served as negative control cells.
- Data are expressed in arbitrary fluorescence units (AFU).
- Figure 3 shows the binding of MV-H antigen preparation to ELISA plates after coating with increasing concentrations of total membrane protein (ng/per well).
- Recombinant H protein was measured using MV-H specific mAb (BH216. Ziegler et al. 1996 J. Gen. Virol. 77:2479-2489) an irrelevant mAb, a positive (HS6111 ) and a negative (HS3071 ) human measles immune serum (HS). Data are shown as net mO.D. measured after 1 hr.
- Figure 6 shows HI and NT titers (expressed as iog2 dilutions) of sera negative by H- ELISA (panel A) or MV-ELISA (panel C) and of sera positive by H-ELISA (B) or MV- sera (D). Numbers (n) of sera are shown.
- Figure 7 shows the standardization of the H-ELISA with dilutions (in dilution buffer) of the 2nd International Standard for anti-measles serum.
- the undiluted Standard contains 5000 mlU.
- the highest concentration tested corresponds to the dilution used for measuring the test sera (1 :300).
- Figure 9 shows the correlation of IgM measured with a certified commercial IgM assay based on whole MV with the H-ELISA. mO.D. of the MV-ELISA below 200 are considered negative. Sera were obtained from acute and convalescent phase measles patients. Both panels show the same individuals using either an enzyme- linked monoclonal antibody specific for human IgM (panel A) or a polyclonal m chain specific conjugate.
- Figure 10 shows a case definition by IgM in MV-ELISA, CDC criteria, or increase in HI, NT and specific IgG levels (found in all paired sera) of 70 measles patients from which single, paired (or multiple) sera were available. For most patients CDC criteria were not evaluated.
- (A) and (B) correspond to patients A and B of Figure 11.
- Panel A displays the moving average based on a period of 4, for H-ELISA (solid line) and MV-ELISA (broken line).
- grey bars represent total number sera tested by H-ELISA and MV-ELISA for each time interval; open and closed bars describe the number of sera tested positive by the MV-ELISA and the H-ELISA, respectively.
- Day 0 corresponds to the day of onset of rash.
- the trendline represents the moving average was based on 4 sera.
- Figure 14B shows IgA versus IgG values by H-ELISA of the sera of panel A (without the 16 negative sera).
- Example 1 Production of recombinant measles virus hemagglutinin protein ( Figure 1 )
- cDNA encoding H protein Three overlapping cDNA fragments (A, B, C) of the MV-H protein were obtained by RT-PCR from total RNA of virus-infected Vero cells (Edmonston strain). They were cloned separately into the pAMPIO vector (pAMPIOAHMV, pAMPIOBHMV, pAMPIOCHMV) by standard cloning techniques. These three cDNA fragments were transferred into the unique BamH I site of pUC-18, to facilitate further manipulations (PUCAMV, PUCBMV, PUCCMV).
- pUC-18 vectors After appropriate digestion of these recombinant pUC-18 vectors, fragments were ligated together to generate a pUC-18 containing the full-length cDNA in its BamH I site (pUC-HMVrev), which was then transferred into the BamH I site of the pSFV1 plasmid (PSFV1-HMV).
- the plasmids were sequenced by asymmetric PCR on a ABI Prism 377 sequencer (Perkin Elmer).
- the full length hemagglutinin cDNA insert was 1857 kb in length, originating from 3 basepairs upstream from the first in-frame AUG, and extending through the stop codon.
- the first basepair (nucleotide A) directly upstream from ATG was changed into a C nucleotide to have an better ribosome binding site (Kozak 1989, J. Cell. Biol.
- Transcription reactions were carried out at 37°C for 1 hr in a 50 ⁇ l volume containing 1-5 ⁇ g of linearized DNA, 40 mM Hepes-KOH (pH7.4), 6 mM MgCI 2 , 2 mM spermidine-HCI, 5 mM dithiothreitol (DTT), 1 mM of ATP, CTP and UTP, 0.5 mM of GTP, 1 mM of m7 G(5')ppp(5')G, 50 units of RNAsin and 30 units of SP6 RNA polymerase.
- RNA was purified by isopropanol precipitation and 1 ml of RNA was analyzed on a 0.5% agarose gel. Parallel transfections were performed with RNA generated from the control plasmid pSFV-lacZ. The latter transfectants served as negative antigen control cells.
- Electroporations were performed as described by Liljestr ⁇ m and Garoff 1995. After trypsinisation, late log-phase cells were washed in PBS (without Mg 2+ or Ca 2+ ) resuspended at 10 7 cells/ml. 800 ml of cells were mixed with the 5-10 ⁇ g RNA purified from the transcription reaction and were transferred to a 0.4 cm chilled electroporation cuvette. Electroporation was carried out at room temperature with two consecutive pulses of 850 kV/25 mF (Bio-Rad Gene Pulser). Cells were then diluted 20-fold in complete medium and transferred back into tissue culture flasks and kept under standard tissue culture conditions. BHK-21 cells transfected with the H- recombinant SFV1 RNA are referred to as BHK-H, control cells mock-transfected with b-galactosidase SFV RNA are called BHK-gal.
- Example 2 Expression and production of hemagglutinin antigen from in vivo - packaged recombinant SFV particles.
- RNA from recombinant pSFV-MVH and the pSFV helper 2 plasmids were performed as described in example 1.
- the two RNA transcripts (mixed in a 1 :1 ratio) were used to transfect BHK-21 cells as described in example 1.
- recombinant RNAs were packaged into SFV particles which are released into the medium. Berglund et al. (1993) BioTechnology 11 : 916-920. 24 hours later, the supernatant was collected and cleared by centrifugation (15 min., 2000xg).
- the recombinant virus initiates only a single round of i ⁇ traceilular replication.
- the titer of the packaged stock cannot be determined by conventional plaque assay, but was tested by indirect immunofluorescence.
- Cells were infected with different dilutions of virus stock and hemagglutinin expression was detected by flow cytometry as described in example 3.
- the supernatant containing the recombinant virus was aliquoted, frozen in liquid nitrogen and stored at -80°C.
- the hemagglutinin recombinant SFV was concentrated and purified from the medium by sucrose gradient centrifugation.
- Medium collected from transfected BHK-21 cells was layered on a sucrose gradient (consisting of 1 ml of 55% sucrose and 3 ml of 20% sucrose) and centrifuged for 90 min.
- the virus was collected from the 20/55% sucrose interphase.
- the medium was aspirated from above with 0.8 ml of the 55% sucrose. From the bottom of the tube recombinant virus was harvested in a total volume of 1 ml and then aliquoted and frozen as described above.
- recombinant virus was activated with 0,5 volume of a-chymotrypsine solution (10 mg/ml PBS and 10 mM MgCI 2 and 20 mM CaCI 2 ; 20 min, room temperature), a-chymotrypsine was inactivated with 0,5 volume of 2 mg/ml of aprotinin. Activated virus was added to washed BHK-21 cells grown to 80% confluency. The infected cells expressed high levels of measles hemagglutinin and their crude membrane extract was an antigen preparation suitable for the detection of measles immunity.
- Transfected cells were harvested after 18 hrs, washed and resuspended in FACS buffer (PBS containing 0.5 % of bovine serum albumin and 0.05% of sodium azide). 50 ml of 10 6 -2x10 6 cells/ml were incubated with dilutions of MV-H specific mAbs. These mAbs included some which recognized conformational dependent epitopes of the native protein, others recognized only denatured protein in its reduced or non- reduced form. Binding of the mAbs was monitored with FITC-conjugated goat anti- mouse IgG antibodies. Cells incubated with an irrelevant mAb or no mAb served as negative controls.
- FACS buffer PBS containing 0.5 % of bovine serum albumin and 0.05% of sodium azide.
- Figure 2 demonstrates that by flow cytometry both a high transfection efficiency (96%) was obtained and that transfected cells expressed high levels of recombinant H protein.
- this example demonstrates that high levels of the recombinant hemagglutinin protein were expressed with high transfection efficiency on the cell surface of transfected BHK-21 cells.
- the protein was indistinguishable from that of the measles virus with regard to its conformational integrity as defined by conformational dependent mAbs and was solely detectable in its native conformation.
- Hemagglutinin transfected BHK-21 cells were also suitable to detect measles virus antibodies in human sera.
- Transfected BHK-21 cells were incubated for 1 hr at 37°C with monkey erythrocytes (100 erythrocytes/BHK cells). Rosette formation was clearly seen in the hemagglutinin transfected BHK-21 cells but not in BHK-21 transfected with RNA from the pSVF1-lacZ which served as a negative control (data not shown). Thus the recombinant H protein exhibit an important functional activity of the measles viral hemagglutinin.
- Monkey erythrocytes were also agglutinated by a suspension of crude membranes derived from hemagglutinin transfected BHK-21 cells and this reaction was inhibited by the addition of sera samples of individuals with measles immunity (data not shown)
- Example 5 Example of a simple preparation of hemagglutinin antigen for the detection of measles hemagglutinin specific antibodies.
- Example 6 Detection of measles hemagglutinin specific IgG by enzyme linked immunosorbant assay using immobilized recombinant hemagglutinin (late convalescents) (Figure 3-7).
- a 05 values were determined.
- the BHK-gal background were 129 ⁇ 21 , 205 ⁇ 41 , 302 ⁇ 68, 353 ⁇ 82 respectively.
- data are expressed as net 90-min mO.D. values by computing for each individual serum or mAb mO.D. (BHK - H > - mO.D. (B H ⁇ -gai).
- BHK - H > - mO.D. (B H ⁇ -gai) In these cells b-galactosidase is produced as a soluble, cytosolic irrelevant protein and mO.D. (BH K-H) /mO.D. ( BH -gai). was always >0.8.
- Sensitivity (%) [true positives / (true positives + false negatives)] x 100
- Negative predictive value (%) (1 - prevalence) x specificity / [ (1 - prevalence) x specificity + (1 - sensitivity) x prevalence] x 100
- the data of Figure 5A was analyzed to determine the number of false positive and false negative sera for both assays. Positivity and negativity was defined on the basis of HI/NT titers.
- Figure 5B focuses only on sera which are double negative for HI/NT (titer ⁇ 1 :2 4 ).
- the corresponding values for the commercial MV-ELISA are defined by the supplier as ⁇ 100 and >200 mO.D.
- a positive serum has 209/212 (98.6 %; one serum being undefined) or a 211/212 (99.5%) chance of being tested positive and a negative serum has an 10/11 (90.9%; one negative serum being undefined) or a 3/11 (27.3 %; two sera being undefined) chance of being tested negative by H-ELISA or MV-ELISA respectively. Since HI is thought to be less sensitive than the NT assay (2, 34, 50), the above analysis based on HI/NT titers potentially excludes weakly positive sera.
- Figure 6 shows the HI/NT values of sera positive or negative for each one of the two ELISAs. Of the sera which were negative by H-ELISA, 10/13 were HI/NT double negative ( Figure 6A).
- Example 7 Detection of measles hemagglutinin specific IgG by enzyme linked immunosorbant assay using immobilized recombinant hemagglutinin (vaccinees) (Figure 8).
- the above assay (example 6) was also used to determine the immunity of measles vaccinees using a panel of sera collected from first year high-school children.
- the H-ELISA was used to determine the immunity of measles vaccinees.
- Table 1 compares the H-ELISA and the MV-ELISA with NT and HI titers respectively.
- the coefficients of determination between H-ELISA and HI or NT titers were considerably higher than those between MV-ELISA and HI or NT.
- the MV-ELISA registered among 10 HI/NT double negative sera 6 as false positive (0/10 vs. 6/10 P ⁇ 0.02).
- the H-ELISA prevails over the MV-ELISA.
- non- responders and seroconverted individuals were most accurately defined with background corrected H-ELISA data. But even when uncorrected O.D. values were used, the assay competed well with the MV-ELISA.
- Example 8 Detection of measles hemaggluinin specific IgM by enzyme linked immunosorbant assay using directly immobilized recombinant hemagglutinin ( Figure 9).
- IgM antibodies For the diagnosis of measles, it is important to detect specific IgM antibodies.
- a panel of sera from acute phase and convalescent phase measles patients were used to test whether the H-antigen preparation described in this invention is also suitable for measuring specific IgM.
- IgM antibodies were detected using an alkaline phosphatase conjugated goat anti human IgM antibody (Figure 9).
- Figure 9 the detection of IgM with a commercial IgM detection assay based on whole MV and with the H-ELISA are compared. The coefficient of determinaton of panel A and B are 0.52 and 0.50 respectively. Sera with mO.D.>200 for the MV-ELISA are considered positive for IgM.
- Figure 9 shows that on the basis of this definition all IgM-positive sera are detected with the H-ELISA (no false negative result) and one (panel A) or two (panel B) sera are false positive.
- Example 9 Detection of measles hemagglutinin specific IgM by ELISA using indirectly coated recombinant hemagglutinin.
- the measles virus hemagglutinin preparation described here was also tested for its suitability to serve as an antigen in an IgM capture ELISA.
- MV-ELISA certified commercial ELISA
- the CDC-criteria include (a) generalized maculopapular rash of 3 days or more; (b) fever of 38.3°C, if measured; (c) at least one of the following symptoms, cough, coryza, or conjunctivitis (Centers for Disease Control 1983 MMWR 31 :707-711.). All patients presented with a typical rash. Four of the 112 samples were obtained between 2 and 14 days before onset of rash; these cases were also confirmed by increased hemagglutination inhibition (HI) test and neutralization (NT) test titers, by MV-specific IgG and IgM antibodies in paired samples drawn after onset of rash.
- HI hemagglutination inhibition
- NT neutralization
- Microtiter plates (Maxisorp, NUNC, Roskilde, Denmark) were coated with 50 ⁇ l of a mixture of three conformational-dependent H-specific monoclonal antibodies (BH81 , BH97, BH125; 5mg/ml) in 0.1 M sodium bicarbonate buffer (pH 9.6).
- the monoclonal antibodies were derived from mice immunized with Edmonston strain MV.
- the plates were washed three times with 1 % Tween 20 in Tris-buffered saline (15 mM, pH 8.0) and incubated for 75 min at room temperature with 50 ⁇ l/well of the above H-antigen (10 mg protein/ml) or negative control antigen.
- the plates were blocked with 1 % bovine serum albumin in Tris-buffered saline (15 mM, pH 7.4).
- Test sera were diluted 1 :10 in Gullsorb (Gull Laboratories, Louvain-La Neuve, Belgium) to eliminate interference of IgG.
- Sera were further diluted to a final dilution of 1 :25 in a modified commercial dilution buffer (Enzymum-test, Boehringer, Mannheim, Germany) and added for 75 min at room temperature to the antigen coated microtiter plates. Plates were washed three times with the above wash buffer.
- Alkaline phosphatase- conjugated goat anti-human IgM (1 :1000; Southern Biotechnology Associates, Birmingham, Ala) and p-nitrophenylphosphate (0.5 mg/ml; 100ml/well) (Sigma, St. Louis, USA) were used to develop the assay.
- Optical density was measured at 405 nm following a 2 hours incubation at 37°C. Data are expressed as milii-optical density (mOD).
- the threshold for positivity was defined as the mean mOD + 2 standard deviations (SD) measured after 2 hours of the IgM-negative sera.
- Experiments with unadsorbed sera gave sometimes false-positive IgM titers in the H-ELISA (data not shown).
- In the present format of the H-ELISA preadsorption with anti-human IgG (GullSORB) gave a more reliable estimation of IgM levels.
- the one serum that was negative in the MV-ELISA was drawn on the day of onset of rash (day 0) and was positive by H-ELISA (372 mOD, patient A in Fig. 11 ). This patient was IgG negative by both ELISAs and developed measles according to CDC criteria.
- a second sample (serum A' in Fig. 11 ) drawn on day 12 from the same patient was IgM positive by both ELISAs (791 and 1142 mOD by MV-ELISA and H- ELISA, respectively).
- This patient experienced a significant increase in HI and NT titers and in specific IgG (6 to 748 mOD by IgG MV-ELISA and 228 to 726 mOD by IgG H-ELISA). This suggests that on day 0 the IgM was accurately measured positive by the H-ELISA, in contrast to the MV-ELISA.
- IgG can be detected in all samples after day 3 (no false negative sample).
- 1013 mOD range 146 to 2076 mOD
- 959 mOD range 215 to 1963 mOD
- H-specific IgM translates into a high sensitivity (98.5%) of the H-ELISA within the first 19 days, which matches that of the Enzygnost MV-ELISA (98.5%) for the same sera.
- sensitivity of the H-ELISA was 92.7% and of the MV-ELISA 98.8%.
- sensitivity between day 0 and 30 was reported to be 91.8% for the Behring test (specificity 98.2%), 93.3% for the Gull test (specificity 90.5%) and 85.5% for the Incstar test (specificity 95.2%) (Arista et al. 1995 Res. Virol. 146:225-232).
- the sensitivity of the H-ELISA rapidly deteriorated (day 0-59: 75%) while the sensitivity of the MV-ELISA did not (98.1 %) because it served as a gold standard.
- the assessment of the sensitivity of the H-ELISA after day 19 may depend on the performance of IgM-Enzygnost. However, essentially no difference in sensitivity of the H-ELISA was found whether the sera were confirmed by the commercial ELISA only (29.4%) or by at least one additional parameter (37.5%). Thus, in our cohort, the difference in sensitivity between the H-ELISA and the MV- ELISA cannot be explained by excessive false positive results (low specificity) of the MV-ELISA, but rather by accelerated waning of H-specific IgM in comparison to MV- IgM.
- the threshold that gave a sensitivity of 98.8% in the H-ELISA was associated with a specificity of 100% in the IgM-negative panel. However, this needs to be confirmed in a panel of IgM-negative sera, which is independent of the definition of the threshold. Lowering the threshold of the H-ELISA would decrease the specificity but increase the sensitivity above 95% within the first 30 days.
- a high specificity, i.e. the low percentage of false positive results was also reported by several authors for the Behring test (Arista et al. 1995 Res. Virol. 146:225-232; Ozanne and d'Halewyn 1992 J. Clin. Microbiol. 30:564-569; Rossier et al. 1991 J. Clin. Microbiol. 29:1069-1071).
- Measles is most contagious within one week before and after onset of rash (Katz 1985 Measles and subacute sclerosing panencephalitis. p. 1062, 18th ed. Appleton- Century-Crofts, New-york, U.S.A.). Serological assays before onset of rash are not available, but during the contagious period after onset of rash the H- and MV-ELISA perform equally well. Most studies which rely on IgM for measles diagnosis recommend serum samples drawn within about 3 weeks after onset of rash (Arista et al. 1995 Res. Virol. 146:225-232; Erdman et al. 1991 J. Clin. Microbiol.
- Example 10 Detection of measles hemagglutinin specific IgA by ELISA using indirectly coated recombinant hemagglutinin.
- Example 9 The assay described in Example 9 was also used to detect IgA using alkaline phosphatase-conjugated goat anti-human IgA (1 :1000, Southern Biotechnology Associates). Essentially the same panel of measles patients was used as in Example 9. In addition, 16 measles virus seronegative donors were used.
- Figure 14A shows that 100% of the IgG seronegative sera were also negative for IgA. Also prior to onset of rash and on day 0-2after onset of rash IgA titers were negative or very low. Later after onset of rash most patients became IgA positive.
- Figure 14B compares the MV-H specific IgG with MV-H specific IgA. These results demonstrate that the H- ELISA also efficiently and reliable detects H-specific IgA. A similar result was obtained when the H protein was directly coated to the microtiter plate.
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FR2935384A1 (en) * | 2008-08-29 | 2010-03-05 | Sysmex Corp | METHOD FOR DETECTING WASTE VIRUS, DEVICE AND KIT USING THE SAME |
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WO1993022683A1 (en) * | 1992-04-24 | 1993-11-11 | The United States Of America, As Represented By The Secretary, Department Of Health And Human Services | Measles virus-specific antibody detection using recombinant measles proteins |
WO1996017072A2 (en) * | 1994-11-30 | 1996-06-06 | Chiron Viagene, Inc. | Recombinant alphavirus vectors |
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WO1993022683A1 (en) * | 1992-04-24 | 1993-11-11 | The United States Of America, As Represented By The Secretary, Department Of Health And Human Services | Measles virus-specific antibody detection using recombinant measles proteins |
WO1996017072A2 (en) * | 1994-11-30 | 1996-06-06 | Chiron Viagene, Inc. | Recombinant alphavirus vectors |
Non-Patent Citations (7)
Title |
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BOUCHE, FABIENNE ET AL: "A simplified immunoassay based on measles virus recombinant hemagglutinin protein for testing the immune status o vaccinees.", JOURNAL OF VIROLOGICAL METHODS, (SEPT., 1998) VOL. 74, NO. 1, PP. 77-87. ISSN: 0166-0934., XP002091976 * |
DRILLIEN R ET AL: "PROTECTION OF MICE FROM FATAL MEASLES ENCEPHALITIS BY VACCINATION WITH VACCINIA VIRUS RECOMBINANTS ENCODING EITHER THE HEMAGGLUTININ OR THE FUSION PROTEIN", PROCEEDINGS OF THE NATIONAL ACADEMY OF SCIENCES OF USA, vol. 85, February 1988 (1988-02-01), pages 1252 - 1256, XP002053143 * |
LILJESTROEM P ET AL: "A NEW GENERATION OF ANIMAL CELL EXPRESSION VECTORS BASED ON THE SEMLIKI FOREST VIRUS REPLICON", BIO/TECHNOLOGY, vol. 9, December 1991 (1991-12-01), pages 1356 - 1361, XP000616021 * |
PAUL, N. L. (1) ET AL: "Expression of HIV-1 envelope glycoproteins by Semliki Forest virus vectors.", AIDS RESEARCH AND HUMAN RETROVIRUSES, (1993) VOL. 9, NO. 10, PP. 963-970. ISSN: 0889-2229., XP002091966 * |
SCHLESINGER S: "ALPHAVIRUSES - VECTORS FOR THE EXPRESSION OF HETEROLOGOUS GENES", TRENDS IN BIOTECHNOLOGY, vol. 11, no. 1, 1 January 1993 (1993-01-01), pages 18 - 22, XP000358625 * |
TAYLOR J ET AL: "NONREPLICATING VIRAL VECTORS AS POTENTIAL VACCINES: RECOMBINANT CANARYPOX VIRUS EXPRESSING MEASLES VIRUS FUSION (F) AND HEMAGGLUTININ (HA) GLYCOPROTEINS", VIROLOGY, vol. 187, no. 1, March 1992 (1992-03-01), pages 321 - 328, XP002053145 * |
TAYLOR J ET AL: "VACCINIA VIRUS RECOMBINANTS EXPRESSING EITHER THE MEASLES VIRUS FUSION OR HEMAGGLUTININ GLYCOPROTEIN PROTECT DOGS AGAINST CANINE DISTEMPER VIRUS CHALLENGE", JOURNAL OF VIROLOGY, vol. 65, no. 8, August 1991 (1991-08-01), pages 4263 - 4274, XP002048181 * |
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FR2935384A1 (en) * | 2008-08-29 | 2010-03-05 | Sysmex Corp | METHOD FOR DETECTING WASTE VIRUS, DEVICE AND KIT USING THE SAME |
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