Showing total 99 results

1. Transfer of proteins from gels to diazobenzyloxymethyl-paper and detection with antisera: a method for studying antibody specificity and antigen structure.

Author

Renart J, Reiser J, and Stark GR

Subjects

Antigens, Viral isolation & purification, Autoradiography, Diazonium Compounds, Electrophoresis, Polyacrylamide Gel, Indicators and Reagents, Proteins isolation & purification, Simian virus 40 immunology, Viral Proteins immunology, Antibody Specificity, Epitopes, Proteins immunology

Abstract

We describe a rapid and very sensitive method for detecting proteins as antigens after their separation in polyacrylamide/agarose composite gels, with or without sodium dodecyl sulfate. The polyacrylamide matrix is crosslinked with a reagent that can be cleaved with periodate or alkali to facilitate transfer of the protein bands to diazobenzyloxymethyl-paper, where they are coupled covalently. Specific proteins are detected by autoradiography after sequential incubation with unfractionated, unlabeled specific antiserum and 125I-labeled protein A from Staphylococcus aureus. Antibody and protein A can be removed with urea and 2-mercaptoethanol, and the same paper can be probed again with a different antiserum. An antiserum specific for the simian virus 40 virion proteins VP3 and VP2 has been prepared; it does not crossreact with VP1, as demonstrated by this method. An antiserum raised in rabbits against simian virus 40-transformed rabbit kidney cells is shown to be directed primarily against a periodate-sensitive moiety present in tumor (T) antigen from infected or transformed cells, whereas an antiserum raised in rabbits against large T antigen purified from lytically infected monkey kidney cells by electrophoresis in the presence of sodium dodecyl sulfate [Lane, D.P. & Robbins, A.K. (1978) Virology 87, 182-193] is directed primarily against determinants that are not sensitive to periodate.

Published

1979

2. Design of immunogens to elicit broadly neutralizing antibodies against HIV targeting the CD4 binding site.

Author

Conti S, Kaczorowski KJ, Song G, Porter K, Andrabi R, Burton DR, Chakraborty AK, and Karplus M

Subjects

AIDS Vaccines chemistry, AIDS Vaccines genetics, Amino Acid Sequence, Antigens, Viral genetics, Antigens, Viral immunology, Binding Sites, Broadly Neutralizing Antibodies chemistry, CD4-Positive T-Lymphocytes chemistry, CD4-Positive T-Lymphocytes immunology, CD4-Positive T-Lymphocytes virology, Crystallography, X-Ray, Epitopes genetics, Epitopes immunology, HIV Antibodies chemistry, HIV Envelope Protein gp120 chemistry, HIV Envelope Protein gp120 genetics, HIV Envelope Protein gp120 metabolism, HIV Envelope Protein gp160 chemistry, HIV Envelope Protein gp160 genetics, HIV Envelope Protein gp160 metabolism, HIV Envelope Protein gp41 chemistry, HIV Envelope Protein gp41 genetics, HIV Envelope Protein gp41 metabolism, HIV Infections immunology, HIV Infections virology, HIV-1 chemistry, HIV-1 genetics, Humans, Models, Molecular, Mutation, Protein Binding, Protein Conformation, alpha-Helical, Protein Conformation, beta-Strand, Protein Engineering methods, Protein Interaction Domains and Motifs, AIDS Vaccines biosynthesis, Antigens, Viral chemistry, Broadly Neutralizing Antibodies biosynthesis, Epitopes chemistry, HIV Antibodies biosynthesis, HIV Infections prevention & control, HIV-1 immunology

Abstract

A vaccine which is effective against the HIV virus is considered to be the best solution to the ongoing global HIV/AIDS epidemic. In the past thirty years, numerous attempts to develop an effective vaccine have been made with little or no success, due, in large part, to the high mutability of the virus. More recent studies showed that a vaccine able to elicit broadly neutralizing antibodies (bnAbs), that is, antibodies that can neutralize a high fraction of global virus variants, has promise to protect against HIV. Such a vaccine has been proposed to involve at least three separate stages: First, activate the appropriate precursor B cells; second, shepherd affinity maturation along pathways toward bnAbs; and, third, polish the Ab response to bind with high affinity to diverse HIV envelopes (Env). This final stage may require immunization with a mixture of Envs. In this paper, we set up a framework based on theory and modeling to design optimal panels of antigens to use in such a mixture. The designed antigens are characterized experimentally and are shown to be stable and to be recognized by known HIV antibodies., Competing Interests: The authors declare no competing interest.

Published

2021

3. TULIP: A transformer-based unsupervised language model for interacting peptides and T cell receptors that generalizes to unseen epitopes.

Author

Meynard-Piganeau, Barthelemy, Feinauer, Christoph, Weigt, Martin, Walczak, Aleksandra M., and Mora, Thierry

Subjects

T cell receptors, LANGUAGE models, TRANSFORMER models, EPITOPES, LANGUAGE acquisition, SUPERVISED learning

Abstract

The accurate prediction of binding between T cell receptors (TCR) and their cognate epitopes is key to understanding the adaptive immune response and developing immunotherapies. Current methods face two significant limitations: the shortage of comprehensive high-quality data and the bias introduced by the selection of the negative training data commonly used in the supervised learning approaches. We propose a method, Transformer-based Unsupervised Language model for Interacting Peptides and T cell receptors (TULIP), that addresses both limitations by leveraging incomplete data and unsupervised learning and using the transformer architecture of language models. Our model is flexible and integrates all possible data sources, regardless of their quality or completeness. We demonstrate the existence of a bias introduced by the sampling procedure used in previous supervised approaches, emphasizing the need for an unsupervised approach. TULIP recognizes the specific TCRs binding an epitope, performing well on unseen epitopes. Our model outperforms state-of-the-art models and offers a promising direction for the development of more accurate TCR epitope recognition models. [ABSTRACT FROM AUTHOR]

Published

2024

4. Natural variation of immune epitopes reveals intrabacterial antagonism.

Author

Stevens, Danielle M., Moreno-Pérez, Alba, Weisberg, Alexandra J., Ramsing, Charis, Fliegmann, Judith, Ning Zhang, Madrigal, Melanie, Martin, Gregory, Steinbrenner, Adam, Felix, Georg, and Coaker, Gitta

Subjects

COLD shock proteins, ELONGATION factors (Biochemistry), BACTERIAL genomes, EPITOPES, PATTERN perception receptors

Abstract

Plants and animals detect biomolecules termed microbe-associated molecular patterns (MAMPs) and induce immunity. Agricultural production is severely impacted by pathogens which can be controlled by transferring immune receptors. However, most studies use a single MAMP epitope and the impact of diverse multicopy MAMPs on immune induction is unknown. Here, we characterized the epitope landscape from five proteinaceous MAMPs across 4,228 plant-associated bacterial genomes. Despite the diversity sampled, natural variation was constrained and experimentally testable. Immune perception in both Arabidopsis and tomato depended on both epitope sequence and copy number variation. For example, Elongation Factor Tu is predominantly single copy, and 92% of its epitopes are immunogenic. Conversely, 99.9% of bacterial genomes contain multiple cold shock proteins, and 46% carry a nonimmunogenic form. We uncovered a mechanism for immune evasion, intrabacterial antagonism, where a nonimmunogenic cold shock protein blocks perception of immunogenic forms encoded in the same genome. These data will lay the foundation for immune receptor deployment and engineering based on natural variation. [ABSTRACT FROM AUTHOR]

Published

2024

5. Stabilized trimeric peptide immunogens of the complete HIV-1 gp41 N-heptad repeat and their use as HIV-1 vaccine candidates.

Author

Chengwei Wu, Raheem, Izzat T., Nahas, Debbie D., Citron, Michael, Kim, Peter S., Montefiori, David C., Ottinger, Elizabeth A., Hepler, Robert W., Hrin, Renee, Patel, Sangita B., Soisson, Stephen M., and Joyce, Joseph G.

Subjects

PEPTIDES, HIV, IMMUNE response, VACCINE development, EPITOPES

Abstract

Efforts to develop an HIV-1 vaccine include those focusing on conserved structural elements as the target of broadly neutralizing monoclonal antibodies. MAb D5 binds to a highly conserved hydrophobic pocket on the gp41 N-heptad repeat (NHR) coiled coil and neutralizes through prevention of viral fusion and entry. Assessment of 17-mer and 36-mer NHR peptides presenting the D5 epitope in rodent immunogenicity studies showed that the longer peptide elicited higher titers of neutralizing antibodies, suggesting that neutralizing epitopes outside of the D5 pocket may exist. Although the magnitude and breadth of neutralization elicited by NHR-targeting antigens are lower than that observed for antibodies directed to other epitopes on the envelope glycoprotein complex, it has been shown that NHR-directed antibodies are potentiated in TZM-bl cells containing the FcγRI receptor. Herein, we report the design and evaluation of covalently stabilized trimeric 51-mer peptides encompassing the complete gp41 NHR. We demonstrate that these peptide trimers function as effective antiviral entry inhibitors and retain the ability to present the D5 epitope. We further demonstrate in rodent and nonhuman primate immunization studies that our 51-mer constructs elicit a broader repertoire of neutralizing antibody and improved cross-clade neutralization of primary HIV-1 isolates relative to 17-mer and 36-mer NHR peptides in A3R5 and FcγR1-enhanced TZM-bl assays. These results demonstrate that sensitive neutralization assays can be used for structural enhancement of moderately potent neutralizing epitopes. Finally, we present expanded trimeric peptide designs which include unique low-molecular-weight scaffolds that provide versatility in our immunogen presentation strategy. [ABSTRACT FROM AUTHOR]

Published

2024

6. Cellular prion protein conformation and function.

Author

Damberger, Fred F., Christen, Barbara, Pérez, Daniel R., Hornemann, Simone, and Wüthrich, Kurt

Subjects

PRIONS, EPITOPES, NUCLEAR magnetic resonance, POLYMORPHISM (Zoology), LABORATORY mice

Abstract

In the otherwise highly conserved NMR structures of cellular prion proteins (PrP~) from different mammals, species variations in a surface epitope that includes a loop linking a β-strand, β2, with a helix, α2, are associated with NMR manifestations of a dynamic equilibrium between locally different conformations. Here, it is shown that this local dynamic conformational polymorphism in mouse PrPC is eliminated through exchange of Tyrl 69 by Ala or Gly, but is preserved after exchange of Tyr 169 with Phe. NMR structure determinations of designed variants of mouse PrP(121-231) at 20°C and of wild-type mPrP(121-231) at 37°C together with analysis of exchange effects on NMR signals then resulted in the identification of the two limiting structures involved in this local conformational exchange in wild-type mouse PrPC, and showed that the two exchanging structures present characteristically different solvent-exposed epitopes near the β2-α2 loop. The structural data presented in this paper provided a platform for currently ongoing, rationally designed experiments with transgenic laboratory animals for, renewed attempts to unravel the so far elusive physiological function of the cellular prion protein. [ABSTRACT FROM AUTHOR]

Published

2011

7. Antigenicity-defined conformations of an extremely neutralization-resistant HIV-1 envelope spike.

Author

Yongfei Cai, Karaca-Griffin, Selen, Jia Chen, Tian, Sai, Fredette, Nicholas, Linton, Christine E., Rits-Volloch, Sophia, Jianming Lu, Kshitij Wagh, Theiler, James, Korber, Bette, Seaman, Michael S., Harrison, Stephen C., Carfi, Andrea, and Bing Chen

Subjects

HIV-1 glycoprotein 120, EPITOPES, NEUTRALIZATION (Chemistry), VIRAL envelope protein structure, MONOCLONAL antibodies

Abstract

The extraordinary genetic diversity of the HIV-1 envelope spike [Env; trimeric (gp160)3, cleaved to (gp120/gp41)3] poses challenges for vaccine development. Envs of different clinical isolates exhibit different sensitivities to antibody-mediated neutralization. Envs of difficult-to-neutralize viruses are thought to be more stable and conformationally homogeneous trimers than those of easyto- neutralize viruses, thereby providing more effective concealment of conserved, functionally critical sites. In this study we have characterized the antigenic properties of an Env derived from one of the most neutralization-resistant HIV-1 isolates, CH120.6. Sequence variation at neutralizing epitopes does not fully account for its exceptional resistance to antibodies. The full-length,membrane-bound CH120.6 Env is indeed stable and conformationally homogeneous. Its antigenicity correlates closely with its neutralization sensitivity, and major changes in antigenicity upon CD4 engagement appear to be restricted to the coreceptor site. The CH120.6 gp140 trimer, the soluble and uncleaved ectodomain of (gp160)3, retains many antigenic properties of the intact Env, consistent with a conformation close to that of Env spikes on a virion, whereas its monomeric gp120 exposes many nonneutralizing or strain-specific epitopes. Thus, trimer organization and stability are important determinants not only for occluding many epitopes but also for conferring resistance to neutralization by all but a small set of antibodies. Env preparations derived from neutralization-resistant viruses may induce irrelevant antibody responses less frequently than do other Envs and may be excellent templates for developing soluble immunogens. [ABSTRACT FROM AUTHOR]

Published

2017

8. MEK inhibition enhances presentation of targetable MHC-I tumor antigens in mutant melanomas.

Author

Stopfer, Lauren E., Rettko, Nicholas J., Leddy, Owen, Mesfin, Joshua M., Brown, Eric, Winski, Shannon, Bryson, Bryan, Wells, James A., and White, Forest M.

Subjects

TUMOR antigens, IMMUNE checkpoint inhibitors, MELANOMA, PEPTIDES, EPITOPES

Abstract

Combining multiple therapeutic strategies in NRAS/BRAF mutant melanoma--namely MEK/BRAF kinase inhibitors, immune checkpoint inhibitors (ICIs), and targeted immunotherapies--may offer an improved survival benefit by overcoming limitations associated with any individual therapy. Still, optimal combination, order, and timing of administration remains under investigation. Here, we measure how MEK inhibition (MEKi) alters anti-tumor immunity by utilizing quantitative immunopeptidomics to profile changes in the peptide major histocompatibility molecules (pMHC) repertoire. These data reveal a collection of tumor antigens whose presentation levels are selectively augmented following therapy, including several epitopes present at over 1,000 copies per cell. We leveraged the tunable abundance of MEKi-modulated antigens by targeting four epitopes with pMHC-specific T cell engagers and antibody drug conjugates, enhancing cell killing in tumor cells following MEK inhibition. These results highlight drug treatment as a means to enhance immunotherapy efficacy by targeting specific upregulated pMHCs and provide a methodological framework for identifying, quantifying, and therapeutically targeting additional epitopes of interest. [ABSTRACT FROM AUTHOR]

Published

2022

9. The neutralizing breadth of antibodies targeting diverse conserved epitopes between SARS-CoV and SARS-CoV-2.

Author

Hualong Xiong, Hui Sun, Siling Wang, Lunzhi Yuan, Liqin Liu, Yuhe Zhu, Jinlei Zhang, Yang Huang, Ruoyao Qi, Yao Jiang, Jian Ma, Ming Zhou, Yue Ma, Rao Fu, Siping Yan, Mingxi Yue, Yangtao Wu, Min Wei, Yizhen Wang, and Tingting Li

Subjects

SARS-CoV-2 Omicron variant, SARS-CoV-2 Delta variant, SARS virus, SARS-CoV-2, EPITOPES, TAX evasion

Abstract

Antibody therapeutics for the treatment of COVID-19 have been highly successful. However, the recent emergence of the Omicron variant has posed a challenge, as it evades detection by most existing SARS-CoV-2 neutralizing antibodies (nAbs). Here, we successfully generated a panel of SARS-CoV-2/SARS-CoV cross-neutralizing antibodies by sequential immunization of the two pseudoviruses. Of the potential candidates, we found that nAbs X01, X10, and X17 offer broad neutralizing potential against most variants of concern, with X17 further identified as a Class 5 nAb with undiminished neutralization against the Omicron variant. Cryo-electron microscopy structures of the three antibodies together in complex with each of the spike proteins of the prototypical SARS-CoV, SARS-CoV-2, and Delta and Omicron variants of SARS-CoV-2 defined three nonoverlapping conserved epitopes on the receptor-binding domain. The triple-antibody mixture exhibited enhanced resistance to viral evasion and effective protection against infection of the Beta variant in hamsters. Our findings will aid the development of antibody therapeutics and broad vaccines against SARS-CoV-2 and its emerging variants. [ABSTRACT FROM AUTHOR]

Published

2022

10. Structural basis for ultrapotent antibody-mediated neutralization of human metapneumovirus.

Author

Banerjee, Avik, Jiachen Huang, Rush, Scott A., Murray, Jackelyn, Gingerich, Aaron D., Royer, Fredejah, Ching-Lin Hsieh, Tripp, Ralph A., McLellan, Jason S., and Mousa, Jarrod J.

Subjects

MONOCLONAL antibodies, HOSPITAL care of children, VIRAL replication, VIRUS diseases, THERAPEUTICS, EPITOPES

Abstract

Human metapneumovirus (hMPV) is a leading cause of morbidity and hospitalization among children worldwide, however, no vaccines or therapeutics are currently available for hMPV disease prevention and treatment. The hMPV fusion (F) protein is the sole target of neutralizing antibodies. To map the immunodominant epitopes on the hMPV F protein, we isolated a panel of human monoclonal antibodies (mAbs), and the mAbs were assessed for binding avidity, neutralization potency, and epitope specificity. We found the majority of the mAbs target diverse epitopes on the hMPV F protein, and we discovered multiple mAb binding approaches for antigenic site III. The most potent mAb, MPV467, which had picomolar potency, was examined in prophylactic and therapeutic mouse challenge studies, and MPV467 limited virus replication in mouse lungs when administered 24 h before or 72 h after viral infection. We determined the structure of MPV467 in complex with the hMPV F protein using cryo-electron microscopy to a resolution of 3.3 Å, which revealed a complex novel prefusion-specific epitope overlapping antigenic sites II and V on a single protomer. Overall, our data reveal insights into the immunodominant antigenic epitopes on the hMPV F protein, identify a mAb therapy for hMPV F disease prevention and treatment, and provide the discovery of a prefusion-specific epitope on the hMPV F protein. [ABSTRACT FROM AUTHOR]

Published

2022

11. Immunosignatures can predict vaccine efficacy.

Author

Barten Legutki, Joseph and Johnston, Stephen Albert

Subjects

VACCINE research, ANTIBODY diversity, PEPTIDES, INFLUENZA viruses, EPITOPES

Abstract

The development of new vaccines would be greatly facilitated by having effective methods to predict vaccine performance. Such methods could also be helpful in monitoring individual vaccine responses to existing vaccines. We have developed "immunosignaturing" as a simple, comprehensive, chip-based method to display the antibody diversity in an individual on peptide arrays. Here we examined whether this technology could be used to develop correlates for predicting vaccine effectiveness. By using a mouse influenza infection, we show that the immunosignaturing of a natural infection can be used to discriminate a protective from nonprotective vaccine. Further, we demonstrate that an immunosignature can determine which mice receiving the same vaccine will survive. Finally, we show that the peptides comprising the correlate signatures of protection can be used to identify possible epitopes in the influenza virus proteome that are correlates of protection. [ABSTRACT FROM AUTHOR]

Published

2013

12. Human T-cell clones used to define functional epitopes on HLA class II molecules.

Author

Weyand CM, Goronzy J, and Fathman CG

Subjects

Antibodies, Monoclonal immunology, Cell Line, Clone Cells, HLA-DQ Antigens, HLA-DR4 Antigen, Haploidy, Humans, Epitopes immunology, Histocompatibility Antigens Class II immunology, T-Lymphocytes immunology

Abstract

Polyclonal reagents have been used to define HLA class II molecules in conventional serologic and cellular typing. We generated human alloreactive T-cell clones to analyze the functional fine specificities of HLA class II molecules that might be important for the phenomenon of HLA and disease association. We chose to examine HLA-Dw14, an HLA-D specificity that has been associated with juvenile rheumatoid arthritis. In this paper we have presented data that suggest that conventional cellular typing does not reflect the distribution of T-cell epitopes on major histocompatibility complex class II molecules. We describe three alloreactive T-cell clones that have defined three separate Dw14-associated T-cell epitopes. Two of these epitopes were on a DR-region molecule; the third was located on a DQ-region product. In a panel of unrelated DR4-positive donors, these three DW14-associated determinants were present in a high frequency but were not linked to each other. Within the tested panel of DR4-positive cells, all possible combinatorial arrangements of these three allodeterminants were seen. The concurrent expression of any two of the three allodeterminants was equivalent to a positive typing response for Dw14. Our finding that HLA-Dw14 is not characterized by a unique allodeterminant but by the combinatorial recognition of independently distributed T-cell interaction sites suggests that analysis of HLA and disease association may be more clearly demonstrated through the use of human T-cell clones.

Published

1986

13. Antibodies specific for NADPH-binding region of enzymes possessing dehydrogenase activities.

Author

Katiyar SS and Porter JW

Subjects

Animals, Binding Sites, Cross Reactions, Fatty Acid Synthases immunology, Folic Acid Antagonists, Glucosephosphate Dehydrogenase immunology, Rabbits, Antibodies immunology, Epitopes analysis, NADP metabolism, Oxidoreductases immunology

Abstract

The results reported in this paper show the presence of a population of antibodies in rabbit polyclonal antiserum that recognize an antigenic site at the NADPH-binding region of enzymes possessing dehydrogenase activities. Antisera from rabbits immunized with glucose-6-phosphate dehydrogenase or fatty acid synthetase were found to inactivate the enzyme dihydrofolate reductase. The inhibitory effect of this site-specific antibody is a time- and concentration-dependent reaction. This immunoinactivation is prevented by preincubation of the enzyme with NADPH.

Published

1983

14. Major histocompatibility complex products restrict the adherence of cytolytic T lymphocytes to minor histocompatibility antigens or to trinitrophenyl determinants on schistosomula of Schistosoma mansoni.

Author

Vadas MA, Butterworth AE, Burakoff S, and Sher A

Subjects

Animals, Antigen-Antibody Reactions, Mice, Mice, Inbred C3H, Mice, Inbred CBA, Mice, Inbred Strains, Epitopes, Histocompatibility Antigens, Isoantibodies, Nitrobenzenes immunology, Schistosoma mansoni immunology, T-Lymphocytes immunology, Trinitrobenzenes immunology

Abstract

We have previously shown that schistosomula passaged through mice acquire histocompatibility (H) antigens that can be recognized either by alloantibody or by alloreactive cytolytic T lymphocytes (CTL). The latter specifically adhere to but fail to damage the parasite. In this paper we describe the use of trinitrophenyl (TNP)-labeled schistosomula to show that the adherence of CTL with specificity for TNP-modified syngeneic cells is restricted by the major histocompatibility complex (MHC) in a fashion similar to that seen in the lysis of TNP-labeled tumor targets. Thus, these CTL adhere only to schistosomula that have both the appropriate H antigens and TNP determinants on their surface, and not to schistosomula bearing either of these antigens by themselves. We note a significant degree of adherence to schistosomula bearing TNP determinants and H antigens allogeneic to the CTL. Anti-minor H antigen CTL are also restricted by the MHC in their adherence; thus, they only adhere to schistosomula that carry both the major and minor H antigens of the stimulator cells. These antigens can be acquired either by a single passage in vivo of schistosomula through congenic strains that possess both the relevant antigens or by sequential passage through two different strains, each contributing one of the antigens in question.

Published

1979

15. Immunochemical analysis of the glucocorticoid receptor: identification of a third domain separate from the steroid-binding and DNA-binding domains.

Author

Carlstedt-Duke J, Okret S, Wrange O, and Gustafsson JA

Subjects

Animals, Binding Sites, Cytosol metabolism, DNA metabolism, Glucocorticoids metabolism, Liver metabolism, Peptide Fragments immunology, Rats, Receptors, Glucocorticoid metabolism, Structure-Activity Relationship, Epitopes analysis, Receptors, Glucocorticoid immunology, Receptors, Steroid immunology

Abstract

The glucocorticoid-receptor complex can be subdivided into three separate domains by limited proteolysis with trypsin or alpha-chymotrypsin. The following characteristics can be separated: steroid-binding activity (domain A), DNA-binding activity (domain B), and immunoactivity (domain C). We have previously reported the separation of the steroid-binding domain from the DNA-binding domain by limited proteolysis of the receptor with trypsin. In this paper, we report the detection by immunochemical analysis of a third domain of the glucocorticoid receptor, which does not bind hormone. Immunoactivity was detected by using specific antiglucocorticoid receptor antibodies raised in rabbits against purified rat liver glucocorticoid receptor and the assay used was an enzyme-linked immunosorbent assay. After digestion with alpha-chymotrypsin, the immunoactive region of the receptor (domain C) was separated from the other two domains (A and B). The immunoactive fragment was found to have a Stokes radius of 2.6 nm. Further digestion with alpha-chymotrypsin resulted in separation of the immunoactive fragment to give a fragment having a Stokes radius of 1.4 nm. The immunoactive domain could be separated from the half of the glucocorticoid receptor containing the steroid-binding and the DNA-binding domains (Stokes radius, 3.3 nm), by limited proteolysis of the receptor by alpha-chymotrypsin followed by gel filtration or chromatography on DNA-cellulose.

Published

1982

16. Codon bias and frequency-dependent selection on the hemagglutinin epitopes of influenza A virus.

Author

Plotkin, Joshua B. and Dushoff, Jonathan

Subjects

*INFLUENZA viruses, *EPITOPES, *HEMAGGLUTININ

Abstract

Although the surface proteins of human influenza A virus evolve rapidly and continually produce antigenic variants, the internal viral genes acquire mutations very gradually. In this paper, we analyze the sequence evolution of three influenza A genes over the past two decades. We study codon usage as a discriminating signature of gene- and even residue-specific diversifying and purifying selection. Nonrandom codon choice can increase or decrease the effective local substitution rate. We demonstrate that the codons of hemagglutinin, particularly those in the antibody-combining regions, are significantly biased toward substitutional point mutations relative to the codons of other influenza virus genes. We discuss the evolutionary interpretation and implications of these biases for hemagglutinin's antigenic evolution. We also introduce information-theoretic methods that use sequence data to detect regions of recent positive selection and potential protein conformational changes. [ABSTRACT FROM AUTHOR]

Published

2003

17. Epistatic models predict mutable sites in SARS-CoV-2 proteins and epitopes.

Author

Rodriguez-Rivas, Juan, Croce, Giancarlo, Muscat, Maureen, and Weigt, Martin

Subjects

SARS-CoV-2, RECEIVER operating characteristic curves, EPITOPES, PROTEIN domains, PROTEIN stability

Abstract

The emergence of new variants of severe acute respiratory syndrome coronavirus 2 (SARS-CoV-2) is a major concern given their potential impact on the transmissibility and pathogenicity of the virus as well as the efficacy of therapeutic interventions. Here, we predict the mutability of all positions in SARS-CoV-2 protein domains to forecast the appearance of unseen variants. Using sequence data from other coronaviruses, preexisting to SARS-CoV-2, we build statistical models that not only capture amino acid conservation but also more complex patterns resulting from epistasis. We show that these models are notably superior to conservation profiles in estimating the already observable SARS-CoV-2 variability. In the receptor binding domain of the spike protein, we observe that the predicted mutability correlates well with experimental measures of protein stability and that both are reliable mutability predictors (receiver operating characteristic areas under the curve ~0.8). Most interestingly, we observe an increasing agreement between our model and the observed variability as more data become available over time, proving the anticipatory capacity of our model. When combined with data concerning the immune response, our approach identifies positions where current variants of concern are highly overrepresented. These results could assist studies on viral evolution and future viral outbreaks and, in particular, guide the exploration and anticipation of potentially harmful future SARS-CoV-2 variants. [ABSTRACT FROM AUTHOR]

Published

2022

18. Mass spectrometric identification of immunogenic SARS-CoV-2 epitopes and cognate TCRs.

Author

Ke Pan, Yulun Chiu, Huang, Eric, Chen, Michelle, Junmei Wang, Ivy Lai, Singh, Shailbala, Shaw, Rebecca M., MacCoss, Michael J., and Yee, Cassian

Subjects

SARS-CoV-2, TANDEM mass spectrometry, EPITOPES, COVID-19 treatment, T cell receptors, COMMERCIAL products

Abstract

Severe acute respiratory syndrome coronavirus 2 (SARS-CoV-2) infections elicit both humoral and cellular immune responses. For the prevention and treatment of COVID-19, the disease caused by SARS-CoV-2, it has become increasingly apparent that T cell responses are equally if not more important than humoral responses in mediating recovery and immune protection. One major challenge in developing T cell-based therapies for infectious and malignant diseases has been the identification of immunogenic epitopes that can elicit a meaningful T cell response. Traditionally, this has been achieved using sophisticated in silico methods to predict putative epitopes deduced from binding affinities. Our studies find that, in contrast to current convention, "immunodominant" SARS-CoV-2 peptides defined by such in silico methods often fail to elicit T cell responses recognizing naturally presented SARS-CoV-2 epitopes. We postulated that immunogenic epitopes for SARS-CoV-2 are best defined empirically by directly analyzing peptides eluted from the naturally processed peptide--major histocompatibility complex (MHC) and then validating immunogenicity by determining whether such peptides can elicit T cells recognizing SARS-CoV-2 antigen-expressing cells. Using a tandem mass spectrometry approach, we identified epitopes derived from not only structural but also nonstructural genes in regions highly conserved among SARS-CoV-2 strains, including recently recognized variants. Finally, there are no reported T cell receptor--engineered T cell technology that can redirect T cell specificity to recognize and kill SARS-CoV-2 target cells. We report here several SARS-CoV-2 epitopes defined by mass spectrometric analysis of MHC-eluted peptides, provide empiric evidence for their immunogenicity, and demonstrate engineered TCR-redirected killing. [ABSTRACT FROM AUTHOR]

Published

2021

19. Influenza hemagglutinin-specific IgA Fc-effector functionality is restricted to stalk epitopes.

Author

Freyn, Alec W., Han, Julianna, Guthmiller, Jenna J., Bailey, Mark J., Neu, Karlynn, Turner, Hannah L., Rosado, Victoria C., Chromikova, Veronika, Min Huang, Strohmeier, Shirin, Liu, Sean T. H., Simon, Viviana, Krammer, Florian, Ward, Andrew B., Palese, Peter, Wilson, Patrick C., and Nachbagauer, Raffael

Subjects

IMMUNOGLOBULIN A, IMMUNOGLOBULIN G, EPITOPES, MONOCLONAL antibodies, FC receptors, COMMERCIAL products

Abstract

In this study, we utilized a panel of human immunoglobulin (Ig) IgA monoclonal antibodies isolated from the plasmablasts of eight donors after 2014/2015 influenza virus vaccination (Fluarix) to study the binding and functional specificities of this isotype. In this cohort, isolated IgA monoclonal antibodies were primarily elicited against the hemagglutinin protein of the H1N1 component of the vaccine. To compare effector functionalities, an H1-specific subset of antibodies targeting distinct epitopes were expressed as monomeric, dimeric, or secretory IgA, as well as in an IgG1 backbone. When expressed with an IgG Fc domain, all antibodies elicited Fc-effector activity in a primary polymorphonuclear cell-based assay which differs from previous observations that found only stalk-specific antibodies activate the low-affinity FcγRIIIa. However, when expressed with IgA Fc domains, only antibodies targeting the stalk domain showed Fceffector activity in line with these previous findings. To identify the cause of this discrepancy, we then confirmed that IgG signaling through the high-affinity FcγI receptor was not restricted to stalk epitopes. Since no corresponding high-affinity Fca receptor exists, the IgA repertoire may therefore be limited to stalk-specific epitopes in the context of Fc receptor signaling. [ABSTRACT FROM AUTHOR]

Published

2021

20. A facile method of mapping HIV-1 neutralizing epitopes using chemically masked cysteines and deep sequencing.

Author

Datta, Rohini, Chowdhury, Rohan Roy, Manjunath, Kavyashree, Hanna, Luke Elizabeth, and Varadarajan, Raghavan

Subjects

ANTIBODY specificity, REVERSE genetics, DISPLAY systems, ANTIBODY formation, EPITOPES

Abstract

Identification of specific epitopes targeted by neutralizing antibodies is essential to advance epitope-based vaccine design strategies. We report a facile methodology for rapid epitope mapping of neutralizing antibodies (NAbs) against HIV-1 Envelope (Env) at single-residue resolution, using Cys labeling, viral neutralization assays, and deep sequencing. This was achieved by the generation of a library of Cys mutations in Env glycoprotein on the viral surface, covalent labeling of the Cys residues using a Cys-reactive label that masks epitope residues, followed by infection of the labeled mutant virions in mammalian cells in the presence of NAbs. Env gene sequencing from NAb-resistant viruses was used to accurately delineate epitopes for the NAbs VRC01, PGT128, and PGT151. These agreed well with corresponding experimentally determined structural epitopes previously inferred from NAb:Env structures. HIV-1 infection is associated with complex and polyclonal antibody responses, typically composed of multiple antibody specificities. Deconvoluting the epitope specificities in a polyclonal response is a challenging task. We therefore extended our methodology to map multiple specificities of epitopes targeted in polyclonal sera, elicited in immunized animals as well as in an HIV-1-infected elite neutralizer capable of neutralizing tier 3 pseudoviruses with high titers. The method can be readily extended to other viruses for which convenient reverse genetics or lentiviral surface display systems are available. [ABSTRACT FROM AUTHOR]

Published

2020

21. Outflanking immunodominance to target subdominant broadly neutralizing epitopes.

Author

Angeletti, Davide, Kosik, Ivan, Santos, Jefferson J. S., Yewdell, William T., Boudreau, Carolyn M., Mallajosyula, Vamsee V. A., Mankowski, Madeleine C., Chambers, Michael, Prabhakaran, Madhu, Hickman, Heather D., McDermott, Adrian B., Alter, Galit, Chaudhuri, Jayanta, and Yewdell, Jonathan W.

Subjects

ANTIBODY formation, INFLUENZA A virus, LYMPH nodes, EPITOPES, HEMAGGLUTININ, VACCINATION

Abstract

A major obstacle to vaccination against antigenically variable viruses is skewing of antibody responses to variable immunodominant epitopes. For influenza virus hemagglutinin (HA), the immunodominance of the variable head impairs responses to the highly conserved stem. Here, we show that head immunodominance depends on the physical attachment of head to stem. Stem immunogenicity is enhanced by immunizing with stem-only constructs or by increasing local HA concentration in the draining lymph node. Surprisingly, coimmunization of full-length HA and stem alters stem-antibody class switching. Our findings delineate strategies for overcoming immunodominance, with important implications for human vaccination. [ABSTRACT FROM AUTHOR]

Published

2019

22. Hypervariable region 1 and N-linked glycans of hepatitis C regulate virion neutralization by modulating envelope conformations.

Author

Prentoe, Jannick, Velázquez-Moctezuma, Rodrigo, Augestad, Elias H., Galli, Andrea, Wang, Richard, Law, Mansun, Alter, Harvey, and Bukh, Jens

Subjects

GLYCANS, HEPATITIS C virus, IMMUNOGLOBULINS, STRUCTURAL dynamics, EPITOPES

Abstract

About two million new cases of hepatitis C virus (HCV) infections annually underscore the urgent need for a vaccine. However, this effort has proven challenging because HCV evades neutralizing antibodies (NAbs) through molecular features of viral envelope glycoprotein E2, including hypervariable region 1 (HVR1) and Nlinked glycans. Here, we observe large variation in the effects of removing individual E2 glycans across HCV strains H77(genotype 1a), J6(2a), and S52(3a) in Huh7.5 cell infections. Also, glycan-mediated effects on neutralization sensitivity were completely HVR1-dependent, and neutralization data were consistent with indirect protection of epitopes, as opposed to direct steric shielding. Indeed, the effect of removing each glycan was similar both in type (protective or sensitizing) and relative strength across four nonoverlapping neutralization epitopes. Temperature-dependent neutralization (e.g., virus breathing) assays indicated that both HVR1 and protective glycans stabilized a closed, difficult to neutralize, envelope conformation. This stabilizing effect was hierarchical as removal of HVR1 fully destabilized closed conformations, irrespective of glycan status, consistent with increased instability at acidic pH and high temperatures. Finally, we observed a strong correlation between neutralization sensitivity and scavenger receptor BI dependency during viral entry. In conclusion, our study indicates that HVR1 and glycans regulate HCV neutralization by shifting the equilibrium between open and closed envelope conformations. This regulation appears tightly linked with scavenger receptor BI dependency, suggesting a role of this receptor in transitions from closed to open conformations during entry. This importance of structural dynamics of HCV envelope glycoproteins has critical implications for vaccine development and suggests that similar phenomena could contribute to immune evasion of other viruses. [ABSTRACT FROM AUTHOR]

Published

2019

23. Oncogenic mutations at the EGFR ectodomain structurally converge to remove a steric hindrance on a kinase-coupled cryptic epitope.

Author

Orellana, Laura, Thorne, Amy H., Lema, Rafael, Gustavsson, Johan, Parisian, Alison D., Hospital, Adam, Cordeiro, Tiago N., Bernadó, Pau, Scott, Andrew M., Brun-Heath, Isabelle, Lindahl, Erik, Cavenee, Webster K., Furnari, Frank B., and Orozco, Modesto

Subjects

GENETIC mutation, EPIDERMAL growth factor receptors, EPITOPES, DELETION mutation, MISSENSE mutation

Abstract

Epidermal growth factor receptor (EGFR) signaling is initiated by a large ligand-favored conformational change of the extracellular domain (ECD) from a closed, self-inhibited tethered monomer, to an open untethered state, which exposes a loop required for strong dimerization and activation. In glioblastomas (GBMs), structurally heterogeneous missense and deletion mutations concentrate at the ECD for unclear reasons. We explore the conformational impact of GBM missense mutations, combining elastic network models (ENMs) with multiple molecular dynamics (MD) trajectories. Our simulations reveal that the main missense class, located at the I-II interface away from the self-inhibitory tether, can unexpectedly favor spontaneous untethering to a compact intermediate state, here validated by smallangle X-ray scattering (SAXS). Significantly, such intermediate is characterized by the rotation of a large ECD fragment (N-TR1), deleted in the most common GBM mutation, EGFRvIII, and that makes accessible a cryptic epitope characteristic of cancer cells. This observation suggested potential structural equivalence of missense and deletion ECD changes in GBMs. Corroborating this hypothesis, our FACS, in vitro, and in vivo data demonstrate that entirely different ECD variants all converge to remove N-TR1 steric hindrance from the 806- epitope, which we show is allosterically coupled to an intermediate kinase and hallmarks increased oncogenicity. Finally, the detected extraintracellular coupling allows for synergistic cotargeting of the intermediate with mAb806 and inhibitors, which is proved herein. [ABSTRACT FROM AUTHOR]

Published

2019

24. Protect, modify, deprotect (PMD): A strategy for creating vaccines to elicit antibodies targeting a specific epitope.

Author

Weidenbacher, Payton A. and Kim, Peter S.

Subjects

IMMUNOGLOBULINS, EPITOPES, IMMUNE response, MONOCLONAL antibodies, HEMAGGLUTININ

Abstract

In creating vaccines against infectious agents, there is often a desire to direct an immune response toward a particular conformational epitope on an antigen.We present amethod, called protect, modify, deprotect (PMD), to generate immunogenic proteins aimed to direct a vaccine-induced antibody (Ab) response toward an epitope defined by a specific monoclonal Ab (mAb). The mAb is used to protect the target epitope on the protein. Then the remaining exposed surfaces of the protein are modified to render them nonimmunogenic. Finally, the epitope is deprotected by removal of the mAb. The resultant protein is modified at surfaces other than the target epitope. We validate PMD using a well-characterized antigen, hen egg white lysozyme, then demonstrate the utility of PMD using influenza virus hemagglutinin (HA). We use an mAb to protect a highly conserved epitope on the stem domain of HA. Exposed surface amines are then modified with short polyethylene glycol chains. The resultant antigen shows markedly reduced binding to mAbs that target the head region of HA, while maintaining binding to mAbs at the epitope of interest. This antigenic preference is also observed with yeast cells displaying Ab fragments. Antisera from guinea pigs immunized with the PMD-modified HA show increased crossreactivity with HAs from other influenza strains, compared with antisera obtainedwith unmodified HA trimers. PMD has the potential to direct an Ab response at high resolution and could be used in combination with other such strategies. There are many attractive targets for the application of PMD. [ABSTRACT FROM AUTHOR]

Published

2019

25. A specific amino acid motif of HLA-DRB1 mediates risk and interacts with smoking history in Parkinson's disease.

Author

Hollenbach, Jill A., Norman, Paul J., Creary, Lisa E., Damotte, Vincent, Montero-Martin, Gonzalo, Caillier, Stacy, Anderson, Kirsten M., Misra, Maneesh K., Nemat-Gorgani, Neda, Kazutoyo Osoegawa, Santaniello, Adam, Renschen, Adam, Marin, Wesley M., Dandekar, Ravi, Parham, Peter, Tanner, Caroline M., Hauser, Stephen L., Fernandez-Viña, Marcelo, and Oksenberg, Jorge R.

Subjects

AMINO acids, PARKINSON'S disease, HLA-DR antigens, GENETIC drift, EPITOPES

Abstract

Parkinson's disease (PD) is a neurodegenerative disease in which genetic risk has been mapped to HLA, but precise allelic associations have been difficult to infer due to limitations in genotyping methodology. Mapping PD risk at highest possible resolution, we performed sequencing of 11 HLA genes in 1,597 PD cases and 1,606 controls. We found that susceptibility to PD can be explained by a specific combination of amino acids at positions 70-74 on the HLADRB1 molecule. Previously identified as the primary risk factor in rheumatoid arthritis and referred to as the “shared epitope" (SE), the residues Q/R-K/R-R-A-A at positions 70-74 in combination with valine at position 11 (11-V) is highly protective in PD, while risk is attributable to the identical epitope in the absence of 11-V. Notably, these effects are modified by history of cigarette smoking, with a strong protective effect mediated by a positive history of smoking in combination with the SE and 11-V (P = 10-4; odds ratio, 0.51; 95% confidence interval, 0.36-0.72) and risk attributable to never smoking in combination with the SE without 11-V (P = 0.01; odds ratio, 1.51; 95% confidence interval, 1.08-2.12). The association of specific combinations of amino acids that participate in critical peptide-binding pockets of the HLA class II molecule implicates antigen presentation in PD pathogenesis and provides further support for genetic control of neuroinflammation in disease. The interaction of HLA-DRB1 with smoking history in disease predisposition, along with predicted patterns of peptide binding to HLA, provide a molecular model that explains the unique epidemiology of smoking in PD. [ABSTRACT FROM AUTHOR]

Published

2019

26. Successive crystal structure snapshots suggest the basis for MHC class I peptide loading and editing by tapasin.

Author

Hafstrand, Ida, Sayitoglu, Ece Canan, Apavaloaei, Anca, Josey, Benjamin John, Renhua Sun, Xiao Han, Pellegrino, Sara, Ozkazanc, Didem, Potens, Renée, Janssen, Linda, Nilvebrant, Johan, Nygren, Per-Åke, Sandalova, Tatyana, Springer, Sebastian, Georgoudaki, Anna-Maria, Duru, Adil Doganay, and Achour, Adnane

Subjects

EPITOPES, ANTIGENS, MAJOR histocompatibility complex, PEPTIDES, CRYSTAL structure, PROTEINS

Abstract

MHC-I epitope presentation to CD8+ T cells is directly dependent on peptide loading and selection during antigen processing. However, the exact molecular bases underlying peptide selection and binding by MHC-I remain largely unknown. Within the peptideloading complex, the peptide editor tapasin is key to the selection of MHC-I-bound peptides. Here, we have determined an ensemble of crystal structures of MHC-I in complex with the peptide exchange-associated dipeptide GL, as well as the tapasin-associated scoop loop, alone or in combination with candidate epitopes. These results combined with mutation analyses allow us to propose a molecular model underlying MHC-I peptide selection by tapasin. The N termini of bound peptides most probably bind first in the N-terminal and middle region of the MHC-I peptide binding cleft, upon which the peptide C termini are tested for their capacity to dislodge the tapasin scoop loop from the F pocket of the MHC-I cleft. Our results also indicate important differences in peptide selection between different MHC-I alleles. [ABSTRACT FROM AUTHOR]

Published

2019

27. HIV peptidome-wide association study reveals patient-specific epitope repertoires associated with HIV control.

Author

Arora, Jatin, McLaren, Paul J., Chaturvedi, Nimisha, Carrington, Mary, Fellay, Jacques, and Lenz, Tobias L.

Subjects

HIV infections, PEPTIDES, HUMAN genetic variation, T cells, EPITOPES

Abstract

Genetic variation in the peptide-binding groove of the highly polymorphic HLA class I molecules has repeatedly been associated with HIV-1 control and progression to AIDS, accounting for up to 12% of the variation in HIV-1 set point viral load (spVL). This suggests a key role in disease control for HLA presentation of HIV-1 epitopes to cytotoxic T cells. However, a comprehensive understanding of the relevant HLA-bound HIV epitopes is still elusive. Here we describe a peptidome-wide association study (PepWAS) approach that integrates HLA genotypes and spVL data from 6,311 HIV-infected patients to interrogate the entire HIV-1 proteome (3,252 unique peptides) for disease-relevant peptides. This PepWAS approach predicts a core set of epitopes associated with spVL, including known epitopes but also several previously uncharacterized disease-relevant peptides. More important, each patient presents only a small subset of these predicted core epitopes through their individual HLA-A and HLA-B variants. Eventually, the individual differences in these patient-specific epitope repertoires account for the variation in spVL that was previously associated with HLA genetic variation. PepWAS thus enables a comprehensive functional interpretation of the robust but little-understood association between HLA and HIV-1 control, prioritizing a short list of diseaseassociated epitopes for the development of targeted therapy. [ABSTRACT FROM AUTHOR]

Published

2019

28. Proinsulin C-peptide is an autoantigen in people with type 1 diabetes.

Author

So, Michelle, Elso, Colleen M., Tresoldi, Eleonora, Pakusch, Miha, Pathiraja, Vimukthi, Wentworth, John M., Harrison, Leonard C., Krishnamurthy, Balasubramanian, Thomas, Helen E., Rodda, Christine, Cameron, Fergus J., McMahon, Jacinta, Kay, Thomas W. H., and Mannering, Stuart I.

Subjects

C-peptide, AUTOANTIGENS, TYPE 1 diabetes, T cells, EPITOPES, IMMUNOTHERAPY

Abstract

Type 1 diabetes (T1D) is an autoimmune disease in which insulin-producing beta cells, found within the islets of Langerhans in the pancreas, are destroyed by islet-infiltrating T cells. Identifying the antigenic targets of beta-cell reactive T cells is critical to gain insight into the pathogenesis of T1D and develop antigen-specific immunotherapies. Several lines of evidence indicate that insulin is an important target of T cells in T1D. Because many human islet-infiltrating CD4+ T cells recognize C-peptide-derived epitopes, we hypothesized that full-length C-peptide (PI33-63), the peptide excised from proinsulin as it is converted to insulin, is a target of CD4+ T cells in people with T1D. CD4+ T cell responses to full-length C-peptide were detected in the blood of: 14 of 23 (>60%) people with recent-onset T1D, 2 of 15 (>13%) people with long-standing T1D, and 1 of 13 (<8%) HLA-matched people without T1D. C-peptide-specific CD4+ T cell clones, isolated from six people with T1D, recognized epitopes from the entire 31 amino acids of C-peptide. Eighty-six percent (19 of 22) of the C-peptide-specific clones were restricted by HLA-DQ8, HLA-DQ2, HLA-DQ8trans, or HLA-DQ2trans, HLA alleles strongly associated with risk of T1D. We also found that full-length C-peptide was a much more potent agonist of some CD4+ T cell clones than an 18mer peptide encompassing the cognate epitope. Collectively, our findings indicate that proinsulin C-peptide is a key target of autoreactive CD4+ T cells in T1D. Hence, full-length C-peptide is a promising candidate for antigen-specific immunotherapy in T1D. [ABSTRACT FROM AUTHOR]

Published

2018

29. Analysis of CD8+ T cell response during the 2013-2016 Ebola epidemic in West Africa.

Author

Saori Sakabe, Sullivan, Brian M., Hartnett, Jessica N., Robles-Sikisaka, Refugio, Gangavarapu, Karthik, Cubitt, Beatrice, Ware, Brian C., Kotliar, Dylan, Branco, Luis M., Goba, Augustine, Momoh, Mambu, Sandi, John Demby, Kanneh, Lansana, Grant, Donald S., Garry, Robert F., Andersen, Kristian G., de la Torre, Juan Carlos, Sabeti, Pardis C., Schieffelin, John S., and Oldstone, Michael B. A.

Subjects

EBOLA virus, EPIDEMICS, IMMUNIZATION, T cells, PATHOGENIC microorganisms

Abstract

The recent Ebola epidemic exemplified the importance of understanding and controlling emerging infections. Despite the importance of T cells in clearing virus during acute infection, little is known about Ebola-specific CD8+ T cell responses. We investigated immune responses of individuals infected with Ebola virus (EBOV) during the 2013-2016 West Africa epidemic in Sierra Leone, where the majority of the >28,000 EBOV disease (EVD) cases occurred. We examined T cell memory responses to seven of the eight Ebola proteins (GP, sGP, NP, VP24, VP30, VP35, and VP40) and associated HLA expression in survivors. Of the 30 subjects included in our analysis, CD8+ T cells from 26 survivors responded to at least one EBOV antigen. A minority, 10 of 26 responders (38%), made CD8+ T cell responses to the viral GP or sGP. In contrast, 25 of the 26 responders (96%) made response to viral NP, 77% to VP24 (20 of 26), 69% to VP40 (18 of 26), 42% (11 of 26) to VP35, with no response to VP30. Individuals making CD8+ T cells to EBOV VP24, VP35, and VP40 also made CD8+ T cells to NP, but rarely to GP. We identified 34 CD8+ T cell epitopes for Ebola. Our data indicate the immunodominance of the EBOV NP-specific T cell response and suggest that its inclusion in a vaccine along with the EBOV GP would best mimic survivor responses and help boost cell-mediated immunity during vaccination. [ABSTRACT FROM AUTHOR]

Published

2018

30. Shared epitope-aryl hydrocarbon receptor crosstalk underlies the mechanism of gene-environment interaction in autoimmune arthritis.

Author

Jiaqi Fu, Nogueira, Sarah V., van Drongelen, Vincent, Coit, Patrick, Song Ling, Rosloniec, Edward F., Sawalha, Amr H., and Holoshitz, Joseph

Subjects

AUTOIMMUNE diseases, RHEUMATOID arthritis, EPITOPES, AMINO acid sequence, ARYL hydrocarbon receptors, NF-kappa B, XENOBIOTICS

Abstract

The susceptibility to autoimmune diseases is affected by genetic and environmental factors. In rheumatoid arthritis (RA), the shared epitope (SE), a five-amino acid sequence motif encoded by RA-associated HLA-DRB1 alleles, is the single most significant genetic risk factor. The risk conferred by the SE is increased in a multiplicative way by exposure to various environmental pollutants, such as cigarette smoke. The mechanism of this synergistic interaction is unknown. It is worth noting that the SE has recently been found to act as a signal transduction ligand that facilitates differentiation of Th17 cells and osteoclasts in vitro and in vivo. Intriguingly, the aryl hydrocarbon receptor (AhR), a transcription factor that mediates the xenobiotic effects of many pollutants, including tobacco combustion products, has been found to activate similar biologic effects. Prompted by these similarities, we sought to determine whether the SE and AhR signaling pathways interact in autoimmune arthritis. Here we uncovered a nuclear factor kappa B-mediated synergistic interaction between the SE and AhR pathways that leads tomarkedly enhanced osteoclast differentiation and Th17 polarization in vitro. Administration of AhR pathway agonists to transgenic mice carrying human SE-coding alleles resulted in a robust increase in arthritis severity, bone destruction, overabundance of osteoclasts, and IL17-expressing cells in the inflamed joints and draining lymph nodes of arthritic mice. Thus, this study identifies a previously unrecognized mechanism of gene- environment interaction that could provide insights into the welldescribed but poorly understood amplification of the genetic risk for RA upon exposure to environmental pollutants. [ABSTRACT FROM AUTHOR]

Published

2018

31. Epitope-specific monoclonal antibodies to FSHβ increase bone mass.

Author

Yaoting Ji, Peng Liu, Yuen, Tony, Haider, Shozeb, Jiahuan He, Romero, Raquel, Hao Chen, Bloch, Madison, Se-Min Kim, Lizneva, Daria, Munshi, Lubna, Chunxue Zhou, Ping Lu, Iqbal, Jameel, Zhen Cheng, New, Maria I., Hsueh, Aaron J., Zhuan Bian, Rosen, Clifford J., and Li Sun

Subjects

FOLLICLE-stimulating hormone, BONE density, EPITOPES, MONOCLONAL antibodies, OSTEOPOROSIS treatment, OBESITY treatment, BONE resorption

Abstract

Pituitary hormones have long been thought solely to regulate single targets. Challenging this paradigm, we discovered that both anterior and posterior pituitary hormones, including FSH, had other functions in physiology. We have shown that FSH regulates skeletal integrity, and, more recently, find that FSH inhibition reduces body fat and induces thermogenic adipose tissue. A polyclonal antibody raised against a short, receptor-binding epitope of FSHß was found not only to rescue bone loss postovariectomy, but also to display marked antiobesity and probeiging actions. Questioning whether a single agent could be used to treat two medical conditions of public health importance--osteoporosis and obesity--we developed two further monoclonal antibodies, Hf2 and Mf4, against computationally defined receptor-binding epitopes of FSHß. Hf2 has already been shown to reduce body weight and fat mass and cause beiging in mice on a high-fat diet. Here, we show that Hf2, which binds mouse Fsh in immunoprecipitation assays, also increases cortical thickness and trabecular bone volume, and microstructural parameters, in sham-operated and ovariectomized mice, noted on microcomputed tomography. This effect was largely recapitulated with Mf4, which inhibited bone resorption by osteoclasts and stimulated new bone formation by osteoblasts. These effects were exerted in the absence of alterations in serum estrogen in wild-type mice. We also reconfirm the existence of Fshrs in bone by documenting the specific binding of fluorescently labeled FSH, FSH-CH, in vivo. Our study provides the framework for the future development of an FSH-based therapeutic that could potentially target both bone and fat. [ABSTRACT FROM AUTHOR]

Published

2018

32. Streamlined circular proximity ligation assay provides high stringency and compatibility with low-affinity antibodies.

Author

Jalili, Roxana, Horecka, Joe, Swartz, James R., Davis, Ronald W., and Persson, Henrik H. J.

Subjects

IMMUNOGLOBULINS, BIOMARKERS, EPITOPES, OLIGONUCLEOTIDES, NANOBIOTECHNOLOGY

Abstract

Proximity ligation assay (PLA) is a powerful tool for quantitative detection of protein biomarkers in biological fluids and tissues. Here, we present the circular proximity ligation assay (c-PLA), a highly specific protein detection method that outperforms traditional PLA in stringency, ease of use, and compatibility with lowaffinity reagents. In c-PLA, two proximity probes bind to an analyte, providing a scaffolding that positions two free oligonucleotides such that they can be ligated into a circular DNA molecule. This assay format stabilizes antigen proximity probe complexes and enhances stringency by reducing the probability of random background ligation events. Circle formation also increases selectivity, since the uncircularized DNA can be removed enzymatically. We compare this method with traditional PLA on several biomarkers and show that the higher stringency for c-PLA improves reproducibility and enhances sensitivity in both buffer and human plasma. The limit of detection ranges from femtomolar to nanomolar concentrations for both methods. Kinetic analyses using surface plasmon resonance (SPR) and biolayer interferometry (BLI) reveal that the variation in limit of detection is due to the variation in antibody affinity and that c-PLA outperforms traditional PLA for low-affinity antibodies. The lower background signal can be used to increase proximity probe concentration while maintaining a high signal-to-noise ratio, thereby enabling the use of low-affinity reagents in a homogeneous assay format. We anticipate that the advantages of c-PLA will be useful in a variety of clinical protein detection applications where high-affinity reagents are lacking. [ABSTRACT FROM AUTHOR]

Published

2018

33. Conserved epitope on influenza-virus hemagglutinin head defined by a vaccine-induced antibody.

Author

Raymond, Donald D., Bajic, Goran, Ferdman, Jack, Suphaphiphat, Pirada, Settembre, Ethan C., Moody, M. Anthony, Schmidt, Aaron G., and Harrison, Stephen C.

Subjects

INFLUENZA vaccines, HEMAGGLUTININ, EPITOPES, INFLUENZA viruses, IMMUNOGLOBULINS, GENETIC mutation, B cells, IMMUNE system

Abstract

Circulating influenza viruses evade neutralization in their human hosts by acquiring escape mutations at epitopes of prevalent antibodies. A goal for next-generation influenza vaccines is to reduce escape likelihood by selectively eliciting antibodies recognizing conserved surfaces on the viral hemagglutinin (HA). The receptor-binding site (RBS) on the HA "head" and a region near the fusion peptide on the HA "stem" are two such sites. We describe here a human antibody clonal lineage' designated CL6649' members of which bind a third conserved site ("lateral patch") on the side of the H1-subtype' HA head. A crystal structure of HA with bound Fab6649 shows the conserved antibody footprint. The site was invariant in isolates from 1977 (seasonal) to 2012 (pdm2009); antibodies in CL6649 recognize HAs from the entire period. In 2013' human H1 viruses acquired mutations in this epitope that were retained in subsequent seasons' prompting modification of the H1 vaccine component in 2017. The mutations inhibit Fab6649 binding. We infer from the rapid spread of these mutations in circulating H1 influenza viruses that the previously subdominant' conserved lateral patch had become immunodominant for individuals with B-cell memory imprinted by earlier H1 exposure. We suggest that introduction of the pdm2009 H1 virus' to which most of the broadly prevalent' neutralizing antibodies did not bind' conferred a selective advantage in the immune systems of infected hosts to recall of memory B cells that recognized the lateral patch' the principal exposed epitope that did not change when pdm2009 displaced previous seasonal H1 viruses. [ABSTRACT FROM AUTHOR]

Published

2018

34. Patterns of conserved gp120 epitope presentation on attached HIV-1 virions.

Author

Mengistu, Meron, Ai-Hui Tang, Foulke Jr., James S., Blanpied, Thomas A., Gonzalez, Mileidy W., Spouge, John L., Gallo, Robert C., Lewis, George K., and Devico, Anthony L.

Subjects

VIRAL envelopes, EPITOPES, MICROSCOPY, VIRION, ELECTRONIC countermeasures, HIV enteropathy

Abstract

A complete picture of HIV antigenicity during early replication is needed to elucidate the full range of options for controlling infection. Such information is frequently gained through analyses of isolated viral envelope antigens, host CD4 receptors, and cognate antibodies. However, direct examination of viral particles and virus-cell interactions is now possible via advanced microscopy techniques and reagents. Using such methods, we recently determined that CD4-induced (CD4i) transition state epitopes in the HIV surface antigen, gp120, while not exposed on free particles, rapidly become immunoreactive upon virus-cell binding. Here, we use 3D direct stochastic optical reconstruction microscopy (dSTORM) to show that certain CD4i epitopes specific to transition state structures are exposed across the surface of cell-bound virions, thus explaining their immunoreactivity. Moreover, such structures and their marker epitopes are dispersed to regions of virions distal to CD4 contact. We further show that the appearance and positioning of distal CD4i exposures is partially dependent on Gag maturation and intact matrix-gp41 interactions within the virion. Collectively, these observations provide a unique perspective of HIV during early replication. These features may define unique insights for understanding how humoral responses target virions and for developing related antiviral countermeasures. [ABSTRACT FROM AUTHOR]

Published

2017

35. Structure of a protective epitope of group B Streptococcus type III capsular polysaccharide.

Author

Carboni, Filippo, Adamo, Roberto, Fabbrini, Monica, De Ricco, Riccardo, Cattaneo, Vittorio, Brogioni, Barbara, Veggi, Daniele, Pinto, Vittoria, Passalacqua, Irene, Oldrini, Davide, Rappuoli, Rino, Malito, Enrico, and Bertia, Francesco

Subjects

STREPTOCOCCUS agalactiae, POLYSACCHARIDES, ANTIBIOTIC prophylaxis, EPITOPES, DEPOLYMERIZATION

Abstract

Despite substantial progress in the prevention of group B Streptococcus (GBS) disease with the introduction of intrapartum antibiotic prophylaxis, this pathogen remains a leading cause of neonatal infection. Capsular polysaccharide conjugate vaccines have been tested in phase I/II clinical studies, showing promise for further development. Mapping of epitopes recognized by protective antibodies is crucial for understanding the mechanism of action of vaccines and for enabling antigen design. In this study, we report the structure of the epitope recognized by a monoclonal antibody with opsonophagocytic activity and representative of the protective response against type III GBS polysaccharide. The structure and the atomic-level interactions were determined by saturation transfer difference (STD)-NMR and X-ray crystallography using oligosaccharides obtained by synthetic and depolymerization procedures. The GBS PSIII epitope is made by six sugars. Four of them derive from two adjacent repeating units of the PSIII backbone and two of them from the branched galactose–sialic acid disaccharide contained in this sequence. The sialic acid residue establishes direct binding interactions with the functional antibody. The crystal structure provides insight into the molecular basis of antibody–carbohydrate interactions and confirms that the conformational epitope is not required for antigen recognition. Understanding the structural basis of immune recognition of capsular polysaccharide epitopes can aid in the design of novel glycoconjugate vaccines. [ABSTRACT FROM AUTHOR]

Published

2017

36. Selective in vivo removal of pathogenic anti-MAG autoantibodies, an antigen-specific treatment option for anti-MAG neuropathy.

Author

Herrendorff, Ruben, Hänggi, Pascal, Pfister, Hélène, Fan Yang, Demeestere, Delphine, Hunziker, Fabienne, Frey, Samuel, Ernst, Beat, Schaeren-Wiemers, Nicole, and Steck, Andreas J.

Subjects

PERIPHERAL neuropathy, IMMUNOGLOBULINS, MYELIN proteins, EPITOPES, AUTOANTIBODIES

Abstract

Anti-MAG (myelin-associated glycoprotein) neuropathy is a disabling autoimmune peripheral neuropathy caused by monoclonal IgM autoantibodies that recognize the carbohydrate epitope HNK-1 (human natural killer-1). This glycoepitope is highly expressed on adhesion molecules, such as MAG, present in myelinated nerve fibers. Because the pathogenicity and demyelinating properties of anti-MAG autoantibodies are well established, current treatments are aimed at reducing autoantibody levels. However, current therapies are primarily immunosuppressive and lack selectivity and efficacy. We therefore hypothesized that a significant improvement in the disease condition could be achieved by selectively neutralizing the pathogenic anti-MAG antibodies with carbohydrate-based ligands mimicking the natural HNK-1 glycoepitope 1. In an inhibition assay, a mimetic (2, mimHNK-1) of the natural HNK-1 epitope blocked the interaction of MAG with pathogenic IgM antibodies from patient sera but with only micromolar affinity. Therefore, considering the multivalent nature of the MAG-IgM interaction, polylysine polymers of different sizes were substituted with mimetic 2. With the most promising polylysine glycopolymer PL84(mimHNK-1)45 the inhibitory effect on patient sera could be improved by a factor of up to 230,000 per epitope, consequently leading to a low-nanomolar inhibitory potency. Because clinical studies indicate a correlation between the reduction of anti-MAG IgM levels and clinical improvement, an immunological surrogate mouse model for anti-MAG neuropathy producing high levels of anti-MAG IgM was developed. The observed efficient removal of these antibodies with the glycopolymer PL84(mimHNK-1)45 represents an important step toward an antigen-specific therapy for anti-MAG neuropathy. [ABSTRACT FROM AUTHOR]

Published

2017

37. Engineered erythrocytes covalently linked to antigenic peptides can protect against autoimmune disease.

Author

Pishesha, Novalia, Bilate, Angelina M., Wibowo, Marsha C., Nai-Jia Huang, Zeyang Li, Dhesycka, Rhogerry, Bousbaine, Djenet, Hojun Li, Patterson, Heide C., Dougan, Stephanie K., Takeshi Maruyama, Lodish, Harvey F., and Ploegh, Hidde L.

Subjects

ERYTHROCYTES, AUTOIMMUNE diseases, IMMUNOSUPPRESSION, ANTIGENS, EPITOPES

Abstract

Current therapies for autoimmune diseases rely on traditional immunosuppressive medications that expose patients to an increased risk of opportunistic infections and other complications. Immunoregulatory interventions that act prophylactically or therapeutically to induce antigen-specific tolerance might overcome these obstacles. Here we use the transpeptidase sortase to covalently attach diseaseassociated autoantigens to genetically engineered and to unmodified red blood cells as a means of inducing antigen-specific tolerance. This approach blunts the contribution to immunity of major subsets of immune effector cells (B cells, CD4+ and CD8+ T cells) in an antigenspecific manner. Transfusion of red blood cells expressing self-antigen epitopes can alleviate and even prevent signs of disease in experimental autoimmune encephalomyelitis, as well as maintain normoglycemia in a mouse model of type 1 diabetes. [ABSTRACT FROM AUTHOR]

Published

2017

38. Multi-institute analysis of carbapenem resistance reveals remarkable diversity, unexplained mechanisms, and limited clonal outbreaks.

Author

Cerqueira, Gustavo C., Earl, Ashlee M., Feldgarden, Michael, Chapman, Sinéad B., Shea, Terrance P., Young, Sarah, Qiandong Zeng, Birren, Bruce W., Wortman, Jennifer R., Murphy, Cheryl I., Ernst, Christoph M., Hung, Deborah T., Grad, Yonatan H., Cosimi, Lisa A., Reis-Cunha, João L., Dekker, John P., Ferraro, Mary Jane, Hooper, David C., Hanage, William P., and Delaney, Mary L.

Subjects

ENTEROBACTERIACEAE, DRUG resistance in bacteria, CARBAPENEMS, BACTERIAL diversity, MOLECULAR evolution, BACTERIAL disease transmission, NUCLEOTIDE sequencing, EPITOPES, BACTERIA

Abstract

Carbapenem-resistant Enterobacteriaceae (CRE) are among the most severe threats to the antibiotic era. Multiple different species can exhibit resistance due to many different mechanisms, and many different mobile elements are capable of transferring resistance between lineages. We prospectively sampled CRE from hospitalized patients from three Boston-area hospitals, together with a collection of CRE from a single California hospital, to define the frequency and characteristics of outbreaks and determine whether there is evidence for transfer of strains within and between hospitals and the frequency with which resistance is transferred between lineages or species. We found eight species exhibiting resistance, with the majority of our sample being the sequence type 258 (ST258) lineage of Klebsiella pneumoniae. There was very little evidence of extensive hospital outbreaks, but a great deal of variation in resistance mechanisms and the genomic backgrounds carrying these mechanisms. Local transmission was evident in clear phylogeographic structure between the samples from the two coasts. The most common resistance mechanisms were KPC (K. pneumoniae carbapenemases) beta-lactamases encoded by blaKPC2, blaKPC3, and blaKPC4, which were transferred between strains and species by seven distinct subgroups of the Tn4401 element. We also found evidence for previously unrecognized resistance mechanisms that produced resistance when transformed into a susceptible genomic background. The extensive variation, together with evidence of transmission beyond limited clonal outbreaks, points to multiple unsampled transmission chains throughout the continuum of care, including asymptomatic carriage and transmission of CRE. This finding suggests that to control this threat, we need an aggressive approach to surveillance and isolation. [ABSTRACT FROM AUTHOR]

Published

2017

39. Structural basis of influenza virus fusion inhibition by the antiviral drug Arbidol.

Author

Kadam, Rameshwar U. and Wilson, Ian A.

Subjects

INFLUENZA viruses, ANTIVIRAL agents, HEMAGGLUTININ, HYDROPHOBIC interactions, EPITOPES, ENDOSOMES, X-ray crystallography

Abstract

The broad-spectrum antiviral drug Arbidol shows efficacy against influenza viruses by targeting the hemagglutinin (HA) fusion machinery. However, the structural basis of the mechanism underlying fusion inhibition by Arbidol has remained obscure, thereby hindering its further development as a specific and optimized influenza therapeutic. We determined crystal structures of Arbidol in complex with influenza virus HA from pandemic 1968 H3N2 and recent 2013 H7N9 viruses. Arbidol binds in a hydrophobic cavity in the HA trimer stem at the interface between two protomers. This cavity is distal to the conserved epitope targeted by broadly neutralizing stem antibodies and is ∼16 Å from the fusion peptide. Arbidol primarily makes hydrophobic interactions with the binding site but also induces some conformational rearrangements to form a network of inter- and intraprotomer salt bridges. By functioning as molecular glue, Arbidol stabilizes the prefusion conformation of HA that inhibits the large conformational rearrangements associated with membrane fusion in the low pH of the endosome. This unique binding mode compared with the small-molecule inhibitors of other class I fusion proteins enhances our understanding of how small molecules can function as fusion inhibitors and guides the development of broad-spectrum therapeutics against influenza virus. [ABSTRACT FROM AUTHOR]

Published

2017

40. Epitope specificity plays a critical role in regulating antibody-dependent cell-mediated cytotoxicity against influenza A virus.

Author

Wenqian He, Tan, Gene S., Mullarkey, Caitlin E., Lee, Amanda J., Wai Lam, Mannie Man, Krammer, Florian, Henry, Carole, Wilson, Patrick C., Ashkar, Ali A., Palese, Peter, and Miller, Matthew S.

Subjects

CELL-mediated cytotoxicity, EPITOPES, INFLUENZA A virus, IMMUNOGLOBULINS, HEMAGGLUTININ, VACCINATION

Abstract

The generation of strain-specific neutralizing antibodies against influenza A virus is known to confer potent protection against homologous infections. The majority of these antibodies bind to the hemagglutinin (HA) head domain and function by blocking the receptor binding site, preventing infection of host cells. Recently, elicitation of broadly neutralizing antibodies which target the conserved HA stalk domain has become a promising "universal" influenza virus vaccine strategy. The ability of these antibodies to elicit Fc-dependent effector functions has emerged as an important mechanism through which protection is achieved in vivo. However, the way in which Fc-dependent effector functions are regulated by polyclonal influenza virus-binding antibody mixtures in vivo has never been defined. Here, we demonstrate that interactions among viral glycoprotein-binding antibodies of varying specificities regulate the magnitude of antibody-dependent cell-mediated cytotoxicity induction. We show that the mechanism responsible for this phenotype relies upon competition for binding to HA on the surface of infected cells and virus particles. Nonneutralizing antibodies were poor inducers and did not inhibit antibody-dependent cell-mediated cytotoxicity. Interestingly, anti-neuraminidase antibodies weakly induced antibody-dependent cell-mediated cytotoxicity and enhanced induction in the presence of HA stalk-binding antibodies in an additive manner. Our data demonstrate that antibody specificity plays an important role in the regulation of ADCC, and that cross-talk among antibodies of varying specificities determines the magnitude of Fc receptor-mediated effector functions. [ABSTRACT FROM AUTHOR]

Published

2016

41. Enhancement of hERG channel activity by scFv antibody fragments targeted to the PAS domain.

Author

Harley, Carol A., Starek, Greg, Jones, David K., Fernandes, Andreia S., Robertson, Gail A., and Morais-Cabral, João H.

Subjects

POTASSIUM channels, LONG QT syndrome, ARRHYTHMIA, SUDDEN death, EPITOPES, ALLOSTERIC regulation

Abstract

The human human ether-à-go-go-related gene (hERG) potassium channel plays a critical role in the repolarization of the cardiac action potential. Changes in hERG channel function underlie long QT syndrome (LQTS) and are associated with cardiac arrhythmias and sudden death. A striking feature of this channel and KCNH channels in general is the presence of an N-terminal Per-Arnt-Sim (PAS) domain. In other proteins, PAS domains bind ligands and modulate effector domains. However, the PAS domains of KCNH channels are orphan receptors. We have uncovered a family of positive modulators of hERG that specifically bind to the PAS domain. We generated two single-chain variable fragments (scFvs) that recognize different epitopes on the PAS domain. Both antibodies increase the rate of deactivation but have different effects on channel activation and inactivation. Importantly, we show that both antibodies, on binding to the PAS domain, increase the total amount of current that permeates the channel during a ventricular action potential and significantly reduce the action potential duration recorded in human cardiomyocytes. Overall, these molecules constitute a previously unidentified class of positive modulators and establish that allosteric modulation of hERG channel function through ligand binding to the PAS domain can be attained. [ABSTRACT FROM AUTHOR]

Published

2016

42. Saturation scanning of ubiquitin variants reveals a common hot spot for binding to USP2 and USP21.

Author

Leung, Isabel, Dekel, Ayelet, Shifman, Julia M., and Sidhu, Sachdev S.

Subjects

SATURATION vapor pressure, MOLECULAR structure of ubiquitin, PROTEASOME inhibitors, EPITOPES, HEMOGLOBIN polymorphisms

Abstract

A detailed understanding of the molecular mechanisms whereby ubiquitin (Ub) recognizes enzymes in the Ub proteasome system is crucial for understanding the biological function of Ub. Many structures of Ub complexes have been solved and, in most cases, reveal a large structural epitope on a common face of the Ub molecule. However, owing to the generally weak nature of these interactions, it has been difficult to map in detail the functional contributions of individual Ub side chains to affinity and specificity. Here we took advantage of Ub variants (Ubvs) that bind tightly to particular Ub-specific proteases (USPs) and used phage display and saturation scanning mutagenesis to comprehensively map functional epitopes within the structural epitopes. We found that Ubvs that bind to USP2 or USP21 contain a remarkably similar core functional epitope, or "hot spot," consisting mainly of positions that are conserved as the wild type sequence, but also some positions that prefer mutant sequences. The Ubv core functional epitope contacts residues that are conserved in the human USP family, and thus it is likely important for the interactions of Ub across many family members. [ABSTRACT FROM AUTHOR]

Published

2016

43. Structural basis for sulfation-dependent self-glycan recognition by the human immune-inhibitory receptor Siglec-8.

Author

Pröpster, Johannes M., Fan Yang, Rabbani, Said, Ernst, Beat, Allain, Frédéric H.-T., and Schubert, Mario

Subjects

LECTINS, GLYCANS, SULFATION, SIALIC acids, NUCLEAR magnetic resonance spectroscopy, IMMUNOREGULATION, INFLAMMATION, EPITOPES

Abstract

Siglec-8 is a human immune-inhibitory receptor that, when engaged by specific self-glycans, triggers eosinophil apoptosis and inhibits mast cell degranulation, providing an endogenous mechanism to down-regulate immune responses of these central inflammatory effector cells. Here we used solution NMR spectroscopy to dissect the fine specificity of Siglec-8 toward different sialylated and sulfated carbohydrate ligands and determined the structure of the Siglec-8 lectin domain in complex with its prime glycan target 6'-sulfo sialyl Lewisx. A canonical motif for sialic acid recognition, extended by a secondary motif formed by unique loop regions, recognizing 6-O-sulfated galactose dictates tight specificity distinct from other Siglec family members and any other endogenous glycan recognition receptors. Structure-guided mutagenesis revealed key contacts of both interfaces to be equally essential for binding. Our work provides critical structural and mechanistic insights into how Siglec-8 selectively recognizes its glycan target, rationalizes the functional impact of site-specific glycan sulfation in modulating this lectin-glycan interaction, and will enable the rational design of Siglec-8-targeted agonists to treat eosinophil- andmast cell-related allergic and inflammatory diseases, such as asthma. [ABSTRACT FROM AUTHOR]

Published

2016

44. Broadly neutralizing epitopes in the Plasmodium vivax vaccine candidate Duffy Binding Protein.

Author

Chen, Edwin, Salinas, Nichole D., Yining Huang, Ntumngia, Francis, Plasencia, Manolo D., Gross, Michael L., Adams, John H., and Tolia, Niraj Harish

Subjects

PLASMODIUM vivax, CARRIER proteins, VACCINES, EPITOPES, X-ray crystallography, X-ray scattering, HYDROGEN-deuterium exchange

Abstract

Plasmodium vivax Duffy Binding Protein (PvDBP) is the most promising vaccine candidate for P. vivax malaria. The polymorphic nature of PvDBP induces strain-specific immune responses, however, and the epitopes of broadly neutralizing antibodies are unknown. These features hamper the rational design of potent DBP-based vaccines and necessitate the identification of globally conserved epitopes. Using X-ray crystallography, small-angle X-ray scattering, hydrogen-deuterium exchange mass spectrometry, and mutational mapping, we have defined epitopes for three inhibitory mAbs (mAbs 2D10, 2H2, and 2C6) and one noninhibitory mAb (3D10) that engage DBP. These studies expand the currently known inhibitory epitope repertoire by establishing protective motifs in subdomain three outside the receptor-binding and dimerization residues of DBP, and introduce globally conserved protective targets. All of the epitopes are highly conserved among DBP alleles. The identification of broadly conserved epitopes of inhibitory antibodies provides critical motifs that should be retained in the next generation of potent vaccines for P. vivax malaria. [ABSTRACT FROM AUTHOR]

Published

2016

45. Heightened self-reactivity associated with selective survival, but not expansion, of naïve virus-specific CD8+ T cells in aged mice.

Author

Quinn, Kylie M., Zaloumis, Sophie G., Cukalac, Tania, Wan-Ting Kan, Sng, Xavier Y. X., Mirams, Michiko, Watson, Katherine A., McCaw, James M., Doherty, Peter C., Thomas, Paul G., Handel, Andreas, and La Gruta, Nicole L.

Subjects

CYTOTOXIC T cells, LYMPHOCYTES, PROTEIN precursors, EPITOPES, CELL proliferation, LABORATORY mice

Abstract

In advanced age, decreased CD8+ cytotoxic T-lymphocyte (CTL) responses to novel pathogens and cancer is paralleled by a decline in the number and function of naïve CTL precursors (CTLp). Although the age-related fall in CD8+ T-cell numbers is well established, neither the underlying mechanisms nor the extent of variation for different epitope specificities have been defined. Furthermore, naïve CD8+ T cells expressing high levels of CD44 accumulate with age, but it is unknown whether this accumulation reflects their preferential survival or an age-dependent driver of CD8+ T-cell proliferation. Here, we track the number and phenotype of four influenza A virus (IAV)- specific CTLp populations in naïve C57BL/6 (B6) mice during aging, and compare T-cell receptor (TCR) clonal diversity for the CD44hi and CD44lo subsets of one such population. We show differential onset of decline for several IAV-specific CD8+ T-cell populations with advanced age that parallel age-associated changes in the B6 immunodominance hierarchy, suggestive of distinct impacts of aging on different epitope-specific populations. Despite finding no evidence of clonal expansions in an aged, epitope-specific TCR repertoire, nonrandom alterations in TCR usage were observed, along with elevated CD5 and CD8 coreceptor expression. Collectively, these data demonstrate that naïve CD8+ T cells expressing markers of heightened selfrecognition are selectively retained, but not clonally expanded, during aging. [ABSTRACT FROM AUTHOR]

Published

2016

46. Reply to van de Sandt and Rimmelzwaan: Matching epitope display with functional avidity.

Author

Keskin, Derin B., Reinhold, Bruce R., Guang Lan Zhang, Ivanov, Alexander R., Karger, Barry L., and Reinherz, Ellis L.

Subjects

INFLUENZA A virus, EPITOPES, CD8 antigen, DIAGNOSIS

Abstract

A response from the authors of the article "Physical detection of influenza A epitopes identifies a stealth subset on human lung epithelium evading natural CD8 immunity" in the 2015 issue is presented.

Published

2015

47. Social relationships and physiological determinants of longevity across the human life span.

Author

Yang Claire Yang, Boen, Courtney, Gerken, Karen, Ting Li, Schorpp, Kristen, and Harris, Kathleen Mullan

Subjects

EPITOPES, LONGITUDINAL method, BIOMARKERS, C-reactive protein, LIFE spans, UNITED States social conditions

Abstract

Two decades of research indicate causal associations between social relationships and mortality, but important questions remain as to how social relationships affect health, when effects emerge, and how long they last. Drawing on data from four nationally representative longitudinal samples of the US population, we implemented an innovative life course design to assess the prospective association of both structural and functional dimensions of social relationships (social integration, social support, and social strain) with objectively measured biomarkers of physical health (C-reactive protein, systolic and diastolic blood pressure, waist circumference, and body mass index) within each life stage, including adolescence and young, middle, and late adulthood, and compare such associations across life stages. We found that a higher degree of social integration was associated with lower risk of physiological dysregulation in a dose- response manner in both early and later life. Conversely, lack of social connections was associated with vastly elevated risk in specific life stages. For example, social isolation increased the risk of inflammation by the same magnitude as physical inactivity in adolescence, and the effect of social isolation on hypertension exceeded that of clinical risk factors such as diabetes in old age. Analyses of multiple dimensions of social relationships within multiple samples across the life course produced consistent and robust associations with health. Physiological impacts of structural and functional dimensions of social relationships emerge uniquely in adolescence and midlife and persist into old age. [ABSTRACT FROM AUTHOR]

Published

2016

48. Rational design of antibodies targeting specific epitopes within intrinsically disordered proteins.

Author

Sormanni, Pietro, Aprile, Francesco A., and Vendruscolo, Michele

Subjects

LIFE sciences, IMMUNOGLOBULINS, EPITOPES, ANTIGENS, SYNUCLEINS

Abstract

Antibodies are powerful tools in life sciences research, as well as in diagnostic and therapeutic applications, because of their ability to bind given molecules with high affinity and specificity. Using current methods, however, it is laborious and sometimes difficult to generate antibodies to target specific epitopes within a protein, in particular if these epitopes are not effective antigens. Here we present a method to rationally design antibodies to enable them to bind virtually any chosen disordered epitope in a protein. The procedure consists in the sequence-based design of one or more complementary peptides targeting a selected disordered epitope and the subsequent grafting of such peptides on an antibody scaffold. We illustrate the method by designing six single-domain antibodies to bind different epitopes within three disease-related intrinsically disordered proteins and peptides (α-synuclein, Aβ42, and IAPP). Our results show that all these designed antibodies bind their targets with good affinity and specificity. As an example of an application, we show that one of these antibodies inhibits the aggregation of α-synuclein at substoichiometric concentrations and that binding occurs at the selected epitope. Taken together, these results indicate that the design strategy that we propose makes it possible to obtain antibodies targeting given epitopes in disordered proteins or protein regions. [ABSTRACT FROM AUTHOR]

Published

2015

49. Generation of MANAbodies specific to HLA-restricted epitopes encoded by somatically mutated genes.

Author

Skora, Andrew D., Douglass, Jacqueline, Hwang, Michael S., Tam, Ada J., Blosser, Richard L., Gabelli, Sandra B., Cao, Jianhong, Diaz Jr., Luis A., Papadopoulos, Nickolas, Kinzler, Kenneth W., Vogelstein, Bert, and Zhou, Shibin

Subjects

HLA histocompatibility antigens, EPITOPES, CANCER genes, IMMUNOGLOBULINS, AMINO acids

Abstract

Mutant epitopes encoded by cancer genes are virtually always located in the interior of cells, making them invisible to conventional antibodies. We here describe an approach to identify single-chain variable fragments (scFvs) specific for mutant peptides presented on the cell surface by HLA molecules. We demonstrate that these scFvs can be successfully converted to full-length antibodies, termed MANAbodies, targeting "Mutation-Associated Neo-Antigens" bound to HLA. A phage display library representing a highly diverse array of single-chain variable fragment sequences was first designed and constructed. A competitive selection protocol was then used to identify clones specific for mutant peptides bound to predefined HLA types. In this way, we obtained two scFvs, one specific for a peptide encoded by a common KRAS mutant and the other by a common epidermal growth factor receptor (EGFR) mutant. The scFvs bound to these peptides only when the peptides were complexed with HLA-A2 (KRAS peptide) or HLA-A3 (EGFR peptide). We converted one scFv to a full-length antibody (MANAbody) and demonstrate that the MANAbody specifically reacts with mutant peptide-HLA complex even when the peptide differs by only one amino acid from the normal, WT form. [ABSTRACT FROM AUTHOR]

Published

2015

50. Two-sided block of a dual-topology F- channel.

Author

Turman, Daniel L., Nathanson, Jacob T., Stockbridge, Randy B., Street, Timothy O., and Miller, Christopher

Subjects

MEMBRANE proteins, ION channels, HOMODIMERS, EPITOPES, TOPOLOGY

Abstract

The Fluc family is a set of small membrane proteins forming F--specific electrodiffusive ion channels that rescue microorganisms from F- toxicity during exposure to weakly acidic environments. The functional channel is built as a dual-topology homodimer with twofold symmetry parallel to the membrane plane. Fluc channels are blocked by nanomolar-affinity fibronectin-domain monobodies originally selected from phage-display libraries. The unusual symmetrical antiparallel dimeric architecture of Flucs demands that the two chemically equivalent monobody-binding epitopes reside on opposite ends of the channel, a double-sided blocking situation that has never before presented itself in ion channel biophysics. However, it is not known if both sites can be simultaneously occupied, and if so,whether monobodies bind independently or cooperatively to their transmembrane epitopes. Here, we use direct monobodybinding assays and single-channel recordings of a Fluc channel homolog to reveal a novel trimolecular blocking behavior that reveals a doubly occupied blocked state. Kinetic analysis of single-channel recordings made with monobody on both sides of the membrane shows substantial negative cooperativity between the two blocking sites. [ABSTRACT FROM AUTHOR]

Published

2015