Login| Sign Up| Help| Contact|

Patent Searching and Data


Title:
METHOD FOR DIFFERENTIATION OF IMMUNE RESPONSE IN AN INDIVIDUAL
Document Type and Number:
WIPO Patent Application WO/2017/089398
Kind Code:
A1
Abstract:
In a first aspect, the present invention relates to a method allowing differentiation between infection-based immune response against an infective agent and a vac- cine induced immune response against an infective agent in an individual. Fur- thermore, a kit or a system is provided allowing differentiation between infection- based immune response against an infective agent and a vaccine induced im- mune response against an infective agent in an individual based on differentiation on antibodies present in the individual directed against linear epitopes and con- formational epitopes. Finally, an array is provided, in particular, a microarray, for multiplex analysis containing different types of antigens.

Inventors:
KRAUSE GÉRARD (DE)
BOHM KATRIN (DE)
SIEVERS CLAUDIA (DE)
Application Number:
PCT/EP2016/078554
Publication Date:
June 01, 2017
Filing Date:
November 23, 2016
Export Citation:
Click for automatic bibliography generation   Help
Assignee:
HELMHOLTZ-ZENTRUM FÜR INFEKTIONSFORSCHUNG GMBH (DE)
International Classes:
G01N33/569; C40B40/02; C40B40/10; G01N33/543; G01N33/68
Domestic Patent References:
WO1999039211A11999-08-05
Other References:
B.-J. HOHLICH ET AL: "Identification of Foot-and-Mouth Disease Virus-Specific Linear B-Cell Epitopes To Differentiate between Infected and Vaccinated Cattle", JOURNAL OF VIROLOGY., vol. 77, no. 16, 15 August 2003 (2003-08-15), US, pages 8633 - 8639, XP055249503, ISSN: 0022-538X, DOI: 10.1128/JVI.77.16.8633-8639.2003
LEWIS S A ET AL: "Expression, processing, and assembly of foot-and-mouth disease virus capsid structures in heterologous systems: Induction of a neutralizing antibody response in guinea pigs", JOURNAL OF VIROLOGY, THE AMERICAN SOCIETY FOR MICROBIOLOGY, US, vol. 65, no. 12, 1 December 1991 (1991-12-01), pages 6572 - 6580, XP002995919, ISSN: 0022-538X
BURBELO P D ET AL: "Antibody-profiling technologies for studying humoral responses to infectious agents", EXPERT REVIEW OF VACCINES, FUTURE DRUGS, LONDON, GB, vol. 9, no. 6, 1 January 2010 (2010-01-01), pages 567 - 578, XP008174047, ISSN: 1476-0584
S. U. EMERSON ET AL: "Identification of VP1/2A and 2C as Virulence Genes of Hepatitis A Virus and Demonstration of Genetic Instability of 2C", JOURNAL OF VIROLOGY., vol. 76, no. 17, 1 September 2002 (2002-09-01), US, pages 8551 - 8559, XP055334801, ISSN: 0022-538X, DOI: 10.1128/JVI.76.17.8551-8559.2002
Attorney, Agent or Firm:
GRAMM, LINS & PARTNER PATENT- UND RECHTSANWÄLTE PARTGMBB (DE)
Download PDF:
Claims:
Claims

An antibody based method for differentiation between infection -based immune response against an infective agent and a vaccine induced immune response against an infective agent in an individual whereby the vaccine is a vaccine based on the infective agent containing an antigen having conformational epitope(s), comprising the steps of:

- providing multiple of antigens derived from the infective agent wherein at least one antigen is provided having a linear epitope and at least one antigen is provided having a conformational epitope whereby the conformational epitope is present in the vaccine;

- allowing formation of binding pairs of an antibody present in a sample obtained from the individual with one of the multiple of antigens provided;

- determining binding pairs of antigen/antibody formed in said sample by an immunological method;

- differentiating infection based immune response and vaccine based immune response against the infective agent i) based on the presence and/or amount of binding pairs of antigen/antibody whereby the antigen has a linear epitope, and ii) based on the presence and/or amount of binding pairs of antigen/antibody whereby the antigen has the conformational epitope;

wherein the determination of the binding pairs is with the same type of immunological method, preferably within a single assay.

The method according to claim 1 wherein the vaccine containing said antigen having conformational epitope(s) is an inactivated or attenuated microorganism, in particular, an inactivated or attenuated whole virus.

The method according to any one of the preceding claims wherein the immunological method is an immunological method selected from multiplex analysis and ELISA.

The method according to any one of the preceding claims wherein the at least one antigen having a linear epitope is at least one recombinant antigen derived from the infective agent.

5. The method according to any one of the preceding claims wherein the infective agent is a virus. 6. The method according to claim 5 wherein the infective agent is a virus selected from hepatitis virus including hepatitis A, hepatitis B, hepatitis C, hepatitis D, hepatitis E, measles virus; rubella virus; mumps virus, influenza virus, human papilloma virus, varicella zoster virus, poliovirus, yellow fever virus, rotavirus, cytomegalovirus, Epstein-Barr- virus, rabies virus.

7. The method according to any one of the preceding claims wherein the immunological method is a multiplex analysis based method, the infective agent is a virus and the vaccine containing the conformational epitope(s) contains inactivated or attenuated virus as active principle.

8. The method according to any one of the preceding claims wherein the number of antigens having a linear epitope is at least two and wherein when no or less than 50% of the antigens having a linear epitope are determined positive for forming a binding pair with antibodies present in the sample of the individual while a binding pair formed of the antigen having a conformational epitope and an antibody present in the sample of the individual is determined, said individual has a vaccine based immune response against the infective agent.

9. The method according to any one of the preceding claims wherein when at least 50% of the antigen having a linear epitope are identified positive for forming a binding pair with antibodies present in the sample of the individual while a binding pair formed of the antigen having a conformational epitope and an antibody present in the sample of the individual is determined, said individual has an infection-based immune response against the infective agent.

10. The method according to any one of the preceding claims wherein the infective agent is a hepatitis virus, like hepatitis A, and the linear antigen is the peptide 2A.

1 1 . A Kit or a system for use in differentiating between infection based immune response against an infective agent and a vaccine induced immune response against an infective agent in an individual, comprising multiple of antigens derived from the infective agent wherein at least one antigen is provided having a linear epitope and at least one antigen is provided having a conformational epitope whereby the conformational epitope is present in the vaccine; means, like antibodies or binding agents binding specifically to the antibodies to be determined for determining antibodies present in a sample of an individual whereby the antibodies are determined as binding pairs of antigens and anti- bodies and whereby said means have optionally a marker moiety for measuring the presence and/or amount of the formed binding pair of antigen/antibody; and, optionally, means for binding the antigens.

12. The kit or system according to claim 1 1 for conducting a method according to any one of claims 1 to 10.

13. The kit or system according to claim 1 1 or 12 wherein the different antigens are present in form of an array, like a microarray, bound to said means in form of microspheres, in particular, coloured microspheres, wherein each antigen is bound to a predetermined type of coloured microspheres.

4. The kit or system according to any one of claims 1 1 to 13 wherein the kit or system is suitable for multiplex analysis, in particular, Luminex based technology.

5. An array, like a microarray, for multiplex analysis, in particular for use in differentiating between infection based immune response against an infective agent and a vaccine induced immune response against an infective agent in an individual containing at least two antigens derived from an infective agent wherein at least one antigen is an antigen having a linear epitope and wherein at least one antigen is an antigen having a conformational epitope of said infective agent, and said array, like said microarray, is a microsphere based array, like a microsphere based microarray.

Description:
Method for differentiation of immune response in an individual

In a first aspect, the present invention relates to a method allowing differentiation between infection-based immune response against an infective agent and a vaccine induced immune response against an infective agent in an individual. Furthermore, a kit or a system is provided allowing differentiation between infection- based immune response against an infective agent and a vaccine induced immune response against an infective agent in an individual based on differentiation on antibodies present in the individual directed against linear epitopes and conformational epitopes. Finally, an array is provided, in particular, a microarray, for multiplex analysis containing different types of antigens.

Prior Art

Human pathogens remain a major public health concern in a society. Specific treatment for viruses is only available for few viruses and increasing spread of antimicrobial and antiviral resistance has developed to a global threat. Undoubtedly the most effective intervention to address this challenge is vaccination. Clinical studies can use conventional immunological biomarkers to measure the effectivity of a new or an established vaccine. Measuring community effectiveness of a vaccination campaign, however, encounters major methodological challenges: 1 ) clinical features of most infections are not pathognomonic enough to allow syndromic measurements as indicator for one unique pathogen, 2) existing immunological markers of vaccine preventable pathogens do not allow the distinction between immunological response to natural infection on one hand and response to vaccination on the other hand. This still remains true for all vaccine preventable pathogens except for hepatitis B, where detection of anti-HBs in absence of HBs-Ag and anti- HBC clearly indicates immunity due to vaccination. Such indicative pattern is not applicable to other vaccine preventable pathogens as of yet. A serological test, able to distinguish between immune response to natural infection and that to vaccination would be of immense benefit for assessing the effectiveness of vaccination strategies. The need for such a tool is particularly urgent in the context of a) epidemics of pathogens with declining sporadic incidence such as Hepatitis A in Europe, b) large vaccination campaigns in a phase of epidemiological transition such as is the case for Hepatitis A in Latin America and c) anticipated introduction of newly developed vaccines such as Hepatitis E in China, d) vaccines of fairly short termed effectivity due to seasonal variations of viral strains with differing antigenic characteristics, as typically know for influenza. By far the most obvious and most ground breaking impact of such a serological tool is to be expected for e) pathogens which are target of global elimination goals, such as measles.

Even the few aforementioned viruses represent a broad scope of species and vaccine designs:

Hepatitis A Virus is a picornavirus, leading to an increasing number of outbreaks in the European Union in recent years and causing a large proportion of hepatic failure among children in various Latin American countries (Tanaka J. (2000) Vaccine, Volume 18, SuppI 1 , 2000, S57-S60). The vaccine currently used is based on an inactivated hepatitis A virus.

Hepatitis E is a yet unclassified RNA virus. WHO estimates 20 million hepatitis E infections with over 3 million symptomatic cases, and 56 600 hepatitis E- related deaths globally. In China a vaccine against HEV has been developed and licensed, which is based on recombinant virus like particles, but still is not included in national vaccination strategies. (. Li, J. Zhang, et a/., (2005) Vaccine, 23, pp. 2893-2901 ).

Influenza viruses are known to cause enormous burden of diseases. The effectiveness of influenza vaccines, currently based on surface antigens (hemagglut- tinin and neuraminidase) of inactivated viruses, are challenged by the seasonal variation or strains and the variability of their respective surface antigens.

Measles, the most prominent and urgent WHO-target for eradication is a paramyxovirus, yearly causing over 100.000 deaths globally. The vaccine is a live attenuated vaccine based on the Edmonston-Enders strain. Mumps is also a paramyxovirus, whose life attenuated form is included in the MMR vaccine, estimated to globally cause over 140.000 deaths every year. Rubella belongs to the togavirus, whose life attenuated form is the third component of the MMR vaccine. The congenital rubella syndrome results in congenital defects or death. WHO estimates that despite widespread vaccination coverage still 100.000 babies are born with CRS every year worldwide.

Existing assays for serological investigations of active infections whereby antibodies are determined can only measure the presence of one type of antibody against said infective agent. That is, the presently available assays allow measuring the presence of one type of antibody only. In addition, the presently available assays do not allow differentiating between infection based immune response against the infective agent and vaccine induced immune response in said individual. However, for determining the level of endemic infection and the success of endemic vaccination, a tool is desired for differentiating natural immune response and vaccine induced immune response in individuals.

That is, for epidemiological studies, e.g. outbreak of infection and level of endemic infection as well as determining the level of vaccination success, screening assays are desired allowing differentiation between these two types of immune response in an individual, in particular, allowing high throughput screening of these individuals at low costs and requiring small amounts of serum.

That is, not only for individual diagnosis of infection, but also in population based serosurveys, these tools and methods may be useful. These methods and tools would be particularly valuable for measuring the impact of recently initiated vaccine campaigns in different parts of the world, e.g. Latin America.

WO 99/3921 1 refers to prognostic allergy or inflammation tests.

Stewart, D.R.S. et al, 1997, The Journal of Infectious Diseases, 176, 593-601 describe the detection of antibodies to the nonstructural 3C proteinase of hepatitis A virus. Therein, it is speculated that use of the 3C proteinase as an antigen can accurately detect antibodies to a non-structural protein and therefore distinguish an immune response to active infection from that resulting from vaccination with an inactivated vaccine since allegedly, the vaccination with inactivated virus should not raise antibodies against the 3C proteinase. However, the present inventors failed to rework the same. Of note, the experiments are based on experimental infection in chimpanzees and not natural infection. Further, Robertson B.H. et al, Journal of Medical Virology, 1993, 40:76-82 describe antibody response to nonstructural proteins of hepatitis A virus following infection. It is discussed therein that the nonstructural proteins of HAV of the P2 region of the viral DNA may be used to differentiate between natural infection and vaccination. It is discussed that the nonstructural proteins may serve as markers for active replication and infection with HAV. Moreover, it is noted that animals immunized with inactivated or life at- tenuated HAV had no evidence of nonstructural antibodies after immunization or challenge with wild type virus. The authors conclude that nonstructural proteins may allow differentiation between inactivated vaccine induced antibodies and natural infection. However, the system is based on in vitro translated structures and the specificity and sensitivity is 87 % and 84 %, respectively only.

Waterboer T. et al, Clin. Chem. 2005, 51 :10, 1845-1853 describe multiplex human papillomavirus serology based on in situ-purified glutathione s-transferase fusion proteins. Therein, a multiplex serology is described enabling antibody analysis of large numbers of sera against up to 100 antigens in parallel having a potential to replace ELISA technology. The technology applied is based on the Luminex technology, namely, the xMAP technology.

Hohlich B.-J. et al., J. Virol., 2003, 77(16) 8633-8639 identifies the identification of foot-and-mouth disease virus-specific linear B-cell epitopes to differentiate between infected and vaccinated cattle. Hohlich et al., teach that only in infected catties linear peptides are reactive while in vaccinated catties, no reactivity against the linear peptides was observed. It is speculated that this allows to differentiate between infected and vaccinated catties.

Lewis S.A. et al., J Virol., 1991 , 65(12), 6572-6580 describes the expression, processing, and assembly of foot-and-mouth disease virus capsid structures in heterologous systems: Induction of a neutralizing antibody response in guinea pigs. This document does not contain any information on differentiation between infection and vaccination based on epitopes.

In Clavijo, A., et al., (2006), Vaccine 24, 1693-1704, simultaneous detection of antibodies to foot-and-mouth disease using non-structural proteins 3ABC, 3D, 3A and 3B by a multiplexed Luminex assay to differentiate infected from vaccinat- ed cattle is described. Therein differentiation should be possible due to the presence or absence of autoantibodies against structural or non-structural proteins. That is, thus far, the approaches are based on the differentiation between structural and non-structural proteins based on the theory that natural infection results in antibodies directed against both, structural and non-structural proteins while vaccine based immune response results in an antibody response against structural proteins only. However, validation of the same failed.

Hence, there is still a need to provide a method and a serological tool for the detection of antibodies allowing differentiation between natural and vaccine based immune response in an individual, thus, allowing identification of the immune response inducing agent.

Brief description of the present invention

In a first aspect, the present invention relates to a method for differentiation between infection-based immune response against an infective agent and a vaccine induced immune response against an infective agent in an individual whereby the vaccine is a vaccine based on the infective agent containing an antigen having conformational epitope(s), comprising the steps of:

providing multiple of antigens derived from the infective agent wherein at least one antigen is provided having a linear epitope and at least one antigen is provided having a conformational epitope whereby the conformational epitope is present in the vaccine;

allowing formation of binding pairs of an antibody present in a sample obtained from the individual with one of the multiple of antigens provided;

- determining binding pairs of antigen/antibody formed in said sample by an immunological method;

differentiating infection based immune response and vaccine based immune response against the infective agent i) based on the presence and/or amount of binding pairs of antigen/antibody whereby the antigen has a linear epitope, and ii) based on the presence and/or amount of binding pairs of antigen/antibody whereby the antigen has the conformational epitope;

wherein the determination of the binding pairs is with the same type of immunological method, preferably within a single assay.

In particular, the method differentiates between an immunization with attenu- ated or inactivated virus and natural infection of said virus.

In a further aspect, the present invention relates to a kit or a system as well as their use for differentiating between infection based immune response against an infective agent and a vaccine induced immune response against an infective agent in an individual, comprising multiple of antigens derived from the infective agent wherein at least one antigen is provided having a linear epitope and at least one antigen is provided having a conformational epitope whereby the conformational epitope is present in the vaccine; means for determining antibodies present in a sample of an individual whereby the antibodies are determined as binding pairs of antigens and antibodies and whereby said means have optionally a marker moiety for measuring the presence and/or amount of the formed binding pair of antigen/antibody; and, optionally, means for binding the antigens.

Finally, the present invention provides an array, like a microarray, for multiplex analysis, containing at least two antigens derived from an infective agent wherein at least one antigen is an antigen having a linear epitope and wherein at least one antigen is an antigen having a conformational epitope of said infective agent, and said array, like said microarray, is a microsphere based array, like a microsphere based microarray and its use in a method according to the present invention.

Brief description of the figures

Figure 1 : The flow chart shows the validation process with which the specific antigen cutoffs as well as the assay cutoff are calculated.

Figure 2: Boxplot for sera with known status in HAV serology. Validation of multiplex serology for the different HAV antigens with negative (0; n = 56), infected (1 ; n = 34) and vaccinated (2; n = 33) serum samples in serum panel 2. Lines across indicate the floating cutoffs for HAV (7.3) and 2A (6.6). The figure shows that only inactivated virus allows the detection of anti-HAV antibodies created by vaccine induced immune response. Moreover 2A showed the best discriminating power in order to differentiate infected sera from either non-infected or vaccinated sera.

Detailed description of the present invention

Reference is made to the priority application EP 15195994.7 which is incorporated by reference herein in full.

In a first aspect, the present invention relates to a method for differentiation between infection-based immune response against an infective agent and vaccine induced immune response against an infective agent in an individual whereby the vaccine is a vaccine based on the infective agent containing an antigen having conformational epitope(s), comprising the steps of:

providing multiple of antigens derived from the infective agent wherein at least one antigen is provided having a linear epitope and at least one antigen is provided having a conformational epitope whereby the conformational epitope is present in the vaccine;

allowing formation of binding pairs of an antibody present in a sample obtained from the individual with one of the multiple of antigens provided;

determining binding pairs of antigen/antibody formed in said sample by an immunological method;

differentiating infection based immune response and vaccine based immune response against the infective agent i) based on the presence and/or amount of binding pairs of antigen/antibody whereby the antigen has a linear epitope, and ii) based on the presence and/or amount of binding pairs of anti- gen/antibody whereby the antigen has the conformational epitope;

wherein the determination of the binding pairs is with the same type of immunological method, preferably within a single assay.

That is, the present inventors recognized that it is possible to differentiate between natural infection, namely, infection based immune response against an infective agent, and vaccine induced or based immune response against an infective agent based on the presence and/or the amount of antibodies recognizing antigen having a linear epitope of the infective agent.

While individuals (either infected or vaccinated) having an immune response against the infective agent have antibodies identifying the antigen with the confor- mational epitope, the type and number of antibodies binding to antigens containing a linear epitope is reduced or for some antigens even absent in the vaccine based immune response in said individual. For example in case of HAV, the infected subjects have antibodies against the linear 2A peptide while the vaccinated subjects do not display any antibody response against said linear 2A peptide. However, the vaccinated subjects may have antibodies directed against other linear epitopes like VP1 or VP2.

Hence, an effective tool is provided for differentiating between natural infection and vaccine induced immune response in an individual. As used herein, the term "virus" refers to whole virus also identified as virus particles and viral vector as well as virus like particles (VLPs). That is, vaccine composition may be composed of virus like particles. Virus like particles are particles resembling viruses but are not infectious because they do not contain any viral genetic material.

Further, the terms "comprise" or "comprising" as well as "contain" or "containing" which are used herein interchangeably include the embodiment of "consist" and "consisting of.

The term "antibody based method" refers to a method including detection of antibodies. That is, an antibody based method may include the embodiment of determining the presence of the antibody by means for binding to antibodies or to antigens bound to said antibodies.

Furthermore, the term "immunological method" refers to a method including the formation of a binding pair composed of antigen/antibody also known as anti- gen/antibody complex.

The present invention is based on the finding that determining antibodies in a sample from an individual directed against linear and conformational epitopes allow to distinguish infected and vaccinated immune response in said individual.

Not to be bound by theory, it is submitted that the vaccine based on inacti- vated or attenuated virus as well as parts of an infective agent being a microorganism is not processed inside the cell upon vaccination which results in a different antibody pattern compared to natural infection. In case of infection, the processing of viral antigens upon the intracellular replication of virus results in antibodies against linear epitopes. Regarding attenuated vaccines, it is submitted that due to the low rate of propagation of said virus, the antibodies directed against linear epitopes are reduced or absent.

In an embodiment, the method of the present invention is a serological method and the samples provided are obtained from blood, in particular in form of a serum, of said individuals to be tested.

In an embodiment of the present invention, the method is a method wherein the vaccine containing said antigen having conformational epitope(s) is an inactivated or attenuated microorganism, in particular, an inactivated or attenuated whole virus. The microorganism may also include bacteria or other infective agents such as protozoa. Further parasites in general are within the scope of vaccine preventbale infective agents.

Of course, the vaccine containing the antigen having conformational epitope(s) may also be a vaccine containing full length antigens derived from the infective agents including diphtheria-toxin, tetanus-toxin, pneumococcus polysaccharides conjugated to carrier proteins, HPV L1 protein or HBV S-antigen.

It is submitted that upon vaccination with these infective agent derived components, including the above mentioned toxins etc., only antibodies against conformational epitopes are produced since the antigens are not processed within infected cells after vaccination.

That is, the virus may be selected from influenza virus, yellow fever virus, human papillomavirus, hepatitis virus, polio virus, rotavirus, rubella virus, measles virus, mumps virus, varicella zoster virus, cytomegalovirus, Epstein-Barr- virus, rabies virus. Hepatitis virus includes hepatitis A virus, hepatitis B virus, hepatitis C virus, hepatitis D virus, hepatitis E virus.

In another embodiment of the present invention, the vaccine is a vaccine based on the infective agent containing said antigen having conformational epitopes including toxoid, polysaccharide present on carrier proteins, as well as surface antigens, in particular diphtheria toxin, tetanus-toxin, pneumococcus poly- saccharides conjugates carrier protein, HPVL1 protein or HBV S-antigen.

In an embodiment of the present invention the virus is hepatitis A virus (HAV) and the linear antigen is the 2A peptide.

In an embodiment of the present invention, the immunological method for determining the binding pairs is conducted in a single assay, e.g. in a multiplex analysis. Suitable example for multiplex analysis or multiplex serology which are used herein interchangeably unless indicated otherwise, include the Luminex technology, e.g. the multiplexing technology platform xMAP. The skilled person is well aware of suitable Luminex assays including the xMAP technology as well as the MagPlex technology of Luminex. These technologies are based on micro- spheres.

As used herein, the term "microspheres" includes the embodiments of beads. Generally, microspheres are small spherical particles with diameters in the micrometre range, typically in the range of 1 μιτι to 1000 μιτι. The microspheres also known as micro-particles include microbeads. The immunological method applied in the method according to the present invention may be a multiplex analysis or an ELISA based analysis. In case of multiplex analysis, the multiplex analysis may be based on microspheres, like the system MagPlex and/or the xMAP technology of Luminex.

In an embodiment of the present invention, the infective agent is a virus, like the virus mentioned above including hepatitis virus, measles virus, rubella virus and mumps virus.

In another embodiment, the at least one antigen having a linear epitope used in the method according to the present invention is a recombinant antigen derived from the infective agent. That is, the antigen is produced recombinantly by known techniques.

Further, an embodiment of the present invention relates to a method wherein the immunological method for determining the binding pairs of antigen antibody, the antigen antibody complex, is a multiplex analysis based method while the in- fective agent is a virus and the vaccine containing the confirmation epitope(s) is an inactivated virus or attenuated virus as active principle.

The multiple of antigens provided in the method according to present invention comprise at least one antigen having a linear epitope and at least one antigen having a conformational epitope whereby the conformational epitope is present in the vaccine. For example, the number of antigens having a linear epitope maybe 2, 3, 4, 5, 6 or even more. In addition, the number of conformational epitopes may be at least 1 , like 2, 3, 4, 5 or 6.

In an embodiment, the number of antigen having a linear epitope are at least 4, like at least 5, as at least 6 while the number of antigen having a conformational epitope is at least 1 .

IN another embodiment, the number of antigen having a linear epitope is 1 antigen, like the 2A antigen in case of HAV or other hepatitis virus and the number of antigen having a conformational epitope is 1 , like inactivated hepatitis A virus or other hepatitis virus.

The skilled person is well aware of suitable buffers and system for providing the multiple of antigens and for performing the steps identified. In particular, the skilled person is well aware of suitable systems including buffer for allowing information of the antigen/antibody complex, namely, the binding pairs of the antibody and antigen as identified. Regarding the determination of the binding pairs, the determination can be effected by known devices typically, based on systems using optical measures like the measurement of mean fluorescence intensities. In addition, the system, e.g. a FACS, may allow determination of the scattered light, thus, allow determination of the size while the laser present in the FACS system allow to determine the formation of the antibody/antigen complex. Alternatively, e.g. using the Luminex system, a dual laser system is used wherein coloured coded beads are present. For each antigen provided, a type of bead is used being specifically colour encoded.

With the immunological method applied, the presence or absence of the binding pair may be determined. In addition, not only the presence or absence but also the level or amount of the formed binding pairs may be determined. Depending on the cutoff value or the threshold value applied, a positive or negative result may be obtained. That is, typically validation of the method according to the present invention may be conducted in so far that references are used with known status, namely, known status regarding natural infection or vaccine based immune response. A cut point is determined, namely, a cutoff or cut point (also known as threshold) allowing to differentiate between a positive result for the natural infection and a negative result for the vaccine based immune response. That is, based on the mean fluorescence intensity, a cut point is set for samples being positive for the antigen and samples being regarded as negative for the antigen, accordingly. This is conducted particularly in case of the antigen having a linear epitope.

In an embodiment of the method according to the present invention, the number of antigens having a linear epitope is at least two and wherein when no or less than 50% of the antigens having a linear epitope are determined positive for forming a binding pair with antibodies present in the sample of the individual while a binding pair is formed of the antigen having a conformational epitope with an antibody present in the sample of the individual, said individual has a vaccine based immune response against the infective agent.

In contrast, when at least 50% of the antigens having a linear epitope are identified positive for forming a binding pair with antibodies present in the sample of the individual while a binding pair formed of the antigen having a conformational epitope with an antibody present in the sample of an individual, said individual has an infection based immune response against the infective agent. In an embodiment, the antigens are provided in a form of an array of said antigens. For example, the antigens may be provided as a microarray of antigens. The skilled person is well aware of suitable kind of arrays. For example, the array may be in form of a protein or peptide microarray. Alternatively, the array may be a mixture of beads having different colour, size and/or density, thus, allowing differentiation with suitable means including FACS and other measuring devices.

In another embodiment, the present invention comprises the step of binding of the different antigens to different types of microspheres including beads. These microspheres may be different between each other based on colour, size or densi- ty.

Determination of bound antibody may be conducted by usual means or measures typically, like antibodies or binding agents binding specifically to the antibodies to be determined. A secondary antibody is used, namely, an anti-human antibody in case of human individuals. The secondary antibody may contain mark- er moieties. That is, commercially available detection systems including these types of antibodies may be used for determining the antigen antibody complexes, namely, the binding pairs mentioned.

With the method according to the present invention simultaneous analysis of antibodies against multiple antigens is possible, thus, allowing measurement of antibody pattern. In addition, measurement of large numbers of serum samples is possible.

In another aspect of the present invention, a kit or system as well as its use for differentiating between infection based immune response against an infective agent and a vaccine induced immune response against an infective agent in an individual, comprising multiple of antigens derived from the infective agent wherein at least one antigen is provided having a linear epitope and at least one antigen is provided having a conformational epitope whereby the conformational epitope is present in the vaccine; means, like antibodies or binding agents binding specifically to the antibodies to be determined, for determining antibodies present in a sam- pie of an individual whereby the antibodies are determined as binding pairs of antigens and antibodies and whereby said means have optionally a marker moiety for measuring the presence and/or amount of the formed binding pair of antigen/antibody; and, optionally, means for binding the antigens is provided. "Means for binding the antigens" refers to molecules or other components allowing binding the antigen on a surface. Examples of said means include microspheres or other activated surfaces, like plastic surfaces. Further, these means may include molecules forming a binding pair with a counterpart present with the antigen, like antibodies or binding pairs like the streptavidin/biotin system.

That is, the kit or system according to the present invention for use in differentiating between infection based immune response and vaccine based immune response in the individual comprise the multiple of antigens. These multiple of antigens may be provided in form of an array, like a microarray. Alternatively, these multiple of antigens may be provided together with means for binding the antigens, e.g. microspheres like beads. Further, said kit or system comprises means for determining antibodies present in a sample of an individual whereby the antibodies are determined as binding pairs of antigens and antibodies. The means include secondary antibodies directed against human antibodies in case the individual is a human. Suitable means are well known to the skilled person. Optionally, these means may contain additionally a marker moiety for measuring the presence and/or amount of the formed binding pair of antigen/antibody. Suitable marker moieties include known label like fluorescence label, radioactive label but also bio- tin, avidin or streptavidin and the like.

The kit or system according to the present invention is useful for conducting a method according to the present invention.

The kit or system is especially adapted for multiplex analysis, in particular, Luminex based technology. That is, the kit or system include microspheres or beads as used in the multiplex analysis, for example, differently coloured beads or differently sized beads. The luminex based technology is well known to the skilled person e.g. exemplified in Burbelo P.D. et al., Expert Rev. Vaccines, 2010, 9(6), 567-578.

Finally, the present invention relates to an array, like a microarray, for multiplex analysis, containing at least two antigens derived from an infective agent wherein at least one antigen is an antigen having a linear epitope and wherein at least one antigen is an antigen having a conformational epitope of said infective agent, and said array, like said microarray, is a microsphere based array, like a microsphere based microarray as well as the use thereof in a method according to the present invention. In case of using a bead mix suitable for the multiplex analysis as described by Luminex, it is possible to determine in one assay antibodies against a multiple of antigens, for example up to 500 antigens, simultaneously. Thereby small amounts of serum is required keeping the costs low.

The present invention provides a valuable tool for efficient population based serosurveys and also for individual differential diagnosis. In particular, the present invention provides a one assay system for differentiation while the prior art requires more than one assay and, even more than one immunological method.

The following examples illustrate the invention further without limiting the same to a specific embodiment described in the examples.

Example 1

Serum

For the validation of the assay we used defined serum samples with known serological HAV status (HAV infected, HAV negative). These samples were provided and IgG status confirmed by the national reference centre for HAV in Re- gensburg, Germany. Serum samples from vaccinated individuals, collected in a study performed at the HZI (ethical approval, # 2198-2014 MHH Hannover, Ger- many), were verified with vaccination card and standard reference ELISA for IgG positivity (Hepatitis A virus Ab ELISA Kit (KA0284, Abnova). HAV status determination done by the reference center and with the Abnova ELISA, respectively are considered as gold standard.

Validation set 1 (antigen cutoff) consisted of 50 anti HAV IgG negative sera and 10 HAV RNA positive sera. Validation set 2 (assay cutoff) consisted of 56 IgG negative samples, 34 IgG positive serum samples of infected individuals and 33 IgG positive serum samples of vaccinated individuals.

Antigens.

The nucleotide sequence NC_001489.1 (NCBI Reference Sequence) for

HAV strain HM175 was used. Full length coding sequences of structural HAV proteins VP1 (bp 2208 - 3107) , VP2 (bp 804 - 1469) and VP3 (bp 1470-2207) and non-structural HAV proteins 2A (bp 3108 - 3674), 2C (3996 - 5000) and 3C (bp 5292 - 5948) were commercially synthesized (MWG) and expressed as double fusion proteins with N-terminal GST and a C-terminal peptide (tag) consisting of the 1 1 C-terminal amino acids from the large T antigen of SV40. The mature peptide without the GST and tag are shown in Seq. ID No. 1 (VP1 ), Seq. ID No. 2 (VP2), Seq. ID No. 3 (VP3), Seq. ID No. 4 (2 A), Seq. ID No. 5 (2C) and Seq. ID No. 6 (3C).The pGex-Tag backbone vector and cloning has been described by Sehr, P. et al. (2001 ) J. Immunol. Methods 253, 153-162. All clones were verified by sequence analysis. Fusion proteins were expressed in E. coli BL21 . Successful full-length antigen expression was verified by Western Blot and anti-tag ELISA as described by Sehr, P. et al. (2001 ) J. Immunol. Methods 253, 153-162.

Glutahione-Casein (GC)

GC was produced as described previously (Sehr, P. et al. (2001 ) J. Immunol. Methods 253, 153-162). Casein (Sigma) at a concentration of 5 mg/ml in phosphate-buffered saline (PBS) was incubated for 15 min at RT with 0.4 mM N- ethylmaleimide (NEM, Sigma) to block the single cysteine residue in casein

Thereafter 4 mM sulfosuccinimidyl 4-[p-maleimidophenyl]butyrate (SSMBP, Pierce, Rockford, IL) was added as crossl inker and the reaction proceeded for 30 min at room temperature. Free SSMBP and NEM were separated from casein by size exclusion chromatography on PD10 columns (GE Healthcare, 17-0851 -01 ) The protein fraction was then supplemented with 10 mM glutathione (Sigma) and the coupling reaction was executed for 1 h at RT. The glutathione casein was separated from unbound glutathione by gel filtration with PD10, using PBS as buffer and stored at -20°C in small aliquots. Covalent Coupling of GC and HAV whole virus to Luminex Microspheres

GC was then coupled to spectrally distinct fluorescence labeled magnetic beads (MagPlex; Luminex) using N-Hydroxysuccinimide and 1 -(3- Dimethylaminopropyl)-3-Ethylcarbodiimide (NHS/EDC) for activation following description by Waterboer, T. et al. (2005) Clin. Chem. 51, 1845-1853. Deviating from the described protocol we used a magnetic separator (Dyna Mag™-2, Life technologies) instead of centrifugation for the washing steps, alternating pelleting of the beads, aspiration of the supernatant and adding 1 ml activation buffer.

Covalent coupling of GC to microspheres allows interchangeable use of microspheres and GST tagged recombinant antigens in bead mix. Whole formalin inactivated HAV virus (Aviva Systems Biology, Cat # OP- MA04543) was coupled to magnetic beads using AMG™ Activation Kit for Multiplex Microspheres according to the manufacturer ' s protocol. Magnetic beads were activated for 1 hour at room temperature with Mix&Go™ activation reagent. Acti- vated magnetic beads were incubated with 200 g formalin inactivated HAV virus for 1 hour at room temperature. HAV coupled magnetic beads can be stored at 4°C in storage buffer.

Multiplex serology.

Multiplex serology (MUSE) was performed as described previously (Water- boer, T. et al. (2005) Clin. Chem. 51, 1845-1853). The complete bead set consisted of beads presenting recombinant antigens and beads coupled with whole inactivated HAV virus. VP1 , VP2, VP3, 2A, 2C and 3C - GST fusion proteins were loaded and affinity-purified on glutathione-casein coupled beads. Serum samples were incubated at 1 :100 final dilution with pooled bead set in 96 well flat bottom plates (Greiner, 655101 ). All plate wash steps were performed with Tecan hydro- flex 96-Well washer (Tecan Austria GmbH). Bound antibodies were quantified with biotinylated goat anti-human IgA, IgM, IgG (Dianova), and R-phycoerythrin- labeled streptavidin (Roche) in a Luminex 100 analyzer as the median R- phycoerythrin fluorescence intensity (MFI) from at least 100 beads of the same bead set.

HAV ELISA

We used Hepatitis A virus Ab ELISA Kit (KA0284, Abnova) for confirmation of antibody status in vaccinated serum samples according to the manufacturer ' s protocol (Gold standard or Reference standard).

Validation.

Antigen-specific MFI values were calculated using a set of standard sera with validated status (Shankar, G., et al. (2008) J. Pharm. Biomed. Anal. 48, 1267- 1281 ). In short, 50 IgG negative serum samples were measured five times in total, by two analysts. After transformation into log scale and exclusion of outliers (+/- 1 .5 IQR) normal distribution was analyzed for all antigens. Mean and variance were estimated using ANOVA. With a same mean a fixed cutoff is calculated for antigens, else a floating cutoff (normalization factor + run specific mean for normalization sera) is used. The antigen specific cutoff is the back transformed mean + 1 .645 Standard deviation (SD). A sample with a MFI > cutoff is positive for the antigen, a samples with a MFI < cutoff negative for the antigen. Validation set 2 was used to calculate the assay cutoff. All statistical analysis was done using SAS 9.2.

HAV Multiplex serology was performed on 50 confirmed anti-HAV-lgG negative sera and the cutoff (mean + 1 .645 SD) and normalization factor, respectively are depicted for each antigen in table 1 .

Results of the statistical evaluation show that a floating cutoff is needed for 5 of the 6 recombinant antigens. The floating cutoff is calculation in each run via the mean of up to ten normalization sera with negative HAV status plus the normalization factor.

A signal above the cutoffs as defined below is considered antibody positive for the respective antigen. Applying HAV multiplex serology on validated infected and vaccinated sera shows that infected sera contain antibodies reactive to in E.coli expressed recombinant viral antigens VP1 - 3C, while vaccinated sera do not react significantly (Figure 1 ).

This result was unexpected as literature results suggested vaccinated and infected sera can be distinguished by showing i) binding of antibodies from both vaccinated and infected serum samples against recombinant structural recombinant proteins (VP1 , VP2, VP3) but only showing ii) binding of antibodies against the non-structural HAV-protease 3C for infected serum. HAV antigens are produced by mammalian cells upon infection. Their expression in E.coli cells can result in incorrect folding. Furthermore, whole virus presents conformational epitopes consisting of amino acid stretches overlapping VP1 , VP2 and VP3, respectively, thus generating epitopes not present on the indi- vidual antigen.

We solved the lacking presentation of conformational epitopes by coupling whole formalin inactivated HAV to magnetic beads. Antibodies from infected serum samples bind with different specificity and sensitivity to the individual recombinant HAV antigens, as seen in table 2.

Table 2: Sensitivity and Specificity for individual recombinant HAV antigens allowing differentiation for HAV negative and infected serum samples, only.

Table 2 Sensitivity and Specificity using the floating cutoff for individual recombinant HAV antigens allowing differentiation for HAV negative and infected serum samples(onlyresults from serum panel 2). n(negative) = 56, n(infected) = 34 and n(vaccinated) = 33). Whole viral particle coupled directly to the beads (HAV virion) detects all anti-HAV IgG/lgA/lgM irrespective of infected (inf.) or vaccinated (vac.) serum status.

HAV antigen 2A by itself is able to distinguish HAV infected from negative sera with a sensitivity and specificity of 88% and 98 %, respectively.

For HAV multiplex serology, the assay cutoff which allows the best differenti- ation between infected, vaccinated and negative serostatus is composed as follows:

Embodiment 1 :

a) Antibody positivity against HAV whole virus and at least any three out of six recombinant antigens is defined as HAV infected serum sample.

b) Antibody positivity against HAV whole virus and maximum any two out of six recombinant antigens is defined as HAV vaccinated serum sample c) Antibody negativity against HAV whole virus is defined as HAV negative serum sample

Embodiment 2: (used in the following)

a) Antibody positivity against HAV whole virus and 2A recombinant antigen is defined as HAV infected serum sample. b) Antibody positivity against HAV whole virus and negative against 2A recombinant antigen is defined as HAV vaccinated serum sample

c) Antibody negativity against HAV whole virus is defined as HAV negative serum sample

Applying the assay cutoff according to embodiment 1 allows the determination of serostatus, as shown in table 3.

Table 3: Sensitivity and Specificity of HAV Multiplex Serology allowing differentiation between HAV negative, infected and vaccinated serum samples based on cutoff embodiment 1 .

Agreement 92.5 %

Result for Validation serum samples using an assay cutoff of 3/6. Any three of the six antigens VP1 , VP2, VP3, 2A, 2C and 3C have to be positive for a serum to be considered 'antigen positive' and therefore 'HAV infected'. A serum positive for HAV whole virus but 'antigen negative' is considered 'HAV vaccinated'. Serum samples 'antigen negative' and HAV whole virus negative are considered HAV negative.

Applying the assay cutoff as defined in embodiment 2 allow the determination fo serostatus as shown in table 4:

Table 4: Sensitivity and Specificity of HAV Multiplex Serology allowing differentiation between HAV negative, infected and vaccinated serum samples based on cut- off embodiment 2. Reference standard

negative infected vaccinated total

negative 19 0 1 20

HAV infected 0 72 6 78

MUSE vaccinated 1 25 74 100

total 20 97 81 198

Table 4 Distribution of serum samples in validation panel 3 according to the reference immune status and the determined status in HAV multiplex serology (HAV MUSE). The sensitivity is 99%, specificity 95% and the accuracy to detect infected individuals is 74% and for vaccinated individuals 91%.

HAV multiplex serology showed a sensitivity of 100% and specificity of 95% to detect anti-HAV IgG/IgM positive individuals. HAV biomarker 2A allowed the differentiation between previously infected and vaccinated individuals. HAV vaccinated individuals could be identified with 91 % accuracy, previously infected individuals with 74% accuracy. Table 5: 381 HAV serum samples used in the validation according to their infection or vaccination status.

HAV status Age group n panel panel panel

1 2 3

HAV IgG negative Adults 126 50 56 20

HAV IgG positive/infected Children 22 - - 22

HAV IgG posiChildren 47 47 tive/vaccinated

HAV IgG posiAdults 67 33 34 tive/vaccinated

HAV IgG positive/infected Adults 75 5 6 64

HAV RNA/lgM positive Adults 44 5 28 1 1

Total 381 60 123 198

Table 5: Distribution of serum samples in validation panel 2 according to the reference immune status and the determined status in HAV multiplex serology (HAV MUSE) following cutoff according to embodiment 2. Definition of HAV virion positive samples as vaccinated and HAV virion and 2A positive samples as HAV infected would result in a sensitivity of 99% and a specificity of 100%. 88% of infected samples and 97% of vaccinated samples would be correctly identified.