Epitope-Specific Human Influenza Antibody Repertoires Diversify by B Cell Intraclonal Sequence Divergence and Interclonal Convergence

Krause, Jens C.; Tsibane, Tshidi; Tumpey, Terrence M.; Huffman, Chelsey J.; Briney, Bryan; Smith, Scott A.; Basler, Christopher F.; Crowe, James E.

doi:10.4049/jimmunol.1101823

Cited by 79 publications

(96 citation statements)

References 42 publications

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“…In addition, within the HA head-specific antibodies, a subgroup of 18 antibodies encoded by V H 3-15 were broadly reactive against former seasonal H1 viruses, whereas the others did not recognize those viruses isolated from at least 1995 to 2007. These patterns and degrees of cross-reactivity between various A viruses and human monoclonal antibodies generated against influenza HA are comparable those found by others (22,23,25,27,28,45,46).…”

Section: Discussionsupporting

confidence: 66%

“…The dominance of HA head-specific V H 3-7*01/J H 6*02 sequences that we found in the largest V H -related set has been seen in other individual responses following exposure to H1N1pdm09 (28,29). For example, the V H 3-7/J H 6 antibodies rearranged with a different group of 4 D segments (3-16*02, 3-22*01, 6-13*01, and 4-17*01) from those from our donor (3-16*01, 3-3*01 in reading frame 2 and 3, and 3-3*02) (28).…”

Section: Discussionmentioning

confidence: 64%

“…For example, the V H 3-7/J H 6 antibodies rearranged with a different group of 4 D segments (3-16*02, 3-22*01, 6-13*01, and 4-17*01) from those from our donor (3-16*01, 3-3*01 in reading frame 2 and 3, and 3-3*02) (28). However, all of these D segments are closely related and share an amino acid sequence motif, DTY, at the D-J junction.…”

Section: Discussionmentioning

confidence: 99%

See 2 more Smart Citations

Focused antibody response to influenza linked to antigenic drift

Huang

Rijal

Schimanski

et al. 2015

Journal of Clinical Investigation

125

139

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Section: Discussionsupporting

confidence: 66%

Section: Discussionmentioning

confidence: 64%

See 1 more Smart Citation

Focused antibody response to influenza linked to antigenic drift

Huang

Rijal

Schimanski

et al. 2015

Journal of Clinical Investigation

125

139

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“…This approach has been used to investigate a variety of phenomena, including effects of influenza vaccination, residual disease in leukemia, effects of immune suppression, and differences between memory and naive B-cell compartments (5)(6)(7)(8)(9)(10)(11).…”

mentioning

confidence: 99%

Genetic measurement of memory B-cell recall using antibody repertoire sequencing

Vollmers

Sit

Weinstein

et al. 2013

Proc. Natl. Acad. Sci. U.S.A.

233

323

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Annual influenza vaccinations aim to protect against seasonal infections, and vaccine strain compositions are updated every year. This protection is based on antibodies that are produced by either newly activated or memory B cells recalled from previous encounters with influenza vaccination or infection. The extent to which the B-cell repertoire responds to vaccination and recalls antibodies has so far not been analyzed at a genetic level-which is to say, at the level of antibody sequences. Here, we developed a consensus read sequencing approach that incorporates unique barcode labels on each starting RNA molecule. These labels allow one to combine multiple sequencing reads covering the same RNA molecule to reduce the error rate to a desired level, and they also enable accurate quantification of RNA and isotype levels. We validated this approach and analyzed the differential response of the antibody repertoire to live-attenuated or trivalent-inactivated influenza vaccination. Additionally, we analyzed the antibody repertoire in response to repeated yearly vaccinations with trivalentinactivated influenza vaccination. We found antibody sequences that were present in both years, providing a direct genetic measurement of B-cell recall.E very year, influenza viruses cause the deaths of an average of 36,000 individuals in the United States alone (1). Although the immunological memory created through vaccination can confer decade-long protection against a particular viral strain, antigenic drift in the original strain and the occurrence of distinct viral strains can enable the virus to evade the immune system (2). As a result, influenza vaccination formulations have to be reevaluated, adjusted, and administered annually to best match the annual influenza strain. Vaccine-induced immunity against influenza is primarily antibody-based, and as such, it relies on the activation of naive B cells or the reactivation (recall) of memory B cells to produce high levels of antibody specific to the vaccine strain. Prior studies approached recall memory responses by measuring plasma antibody levels and specificity or sequencing antibody loci of isolated B cells, with one study concluding that the response to influenza vaccination is pauciclonal (i.e., composed of only a few distinct clones) (3, 4). However, this study and others were limited in the number of B cells that they were able to analyze and not able to show that the same clone recurs during recall. The strength of the recall response, the isotype distribution, and the clonal relationship to others have been unclear.Recently, methods to sequence antibody repertoires of whole organisms and human blood samples were developed and applied to investigate several features of B-cell repertoires (5, 6). This approach has been used to investigate a variety of phenomena, including effects of influenza vaccination, residual disease in leukemia, effects of immune suppression, and differences between memory and naive B-cell compartments (5-11).Analyzing vaccine recall response requires ...

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“…There are several methods for isolation, amplification, and sequencing of B-cell repertoires. Multiplex PCR amplification, using degenerate PCR primers complementary to germ-line V and J segments have been designed and validated previously (van Dongen et al 2003;Lukowsky et al 2006;Bruggemann et al 2007;Evans et al 2007;van Krieken et al 2007; Vargas et al 2008), used in numerous biological studies (Sanchez et al 2003;Campbell et al 2008;Boyd et al 2009Boyd et al , 2010Krause et al 2011;Jager et al 2012;Lev et al 2012;Maletzki et al 2012), and optimized for clinical use (McClure et al 2006;Harris et al 2012;Sproul and Goodlad 2012), although the potential for biased PCR amplification remains. The 59 rapid amplification of cDNA ends (59 RACE) has also been used (Bertioli 1997;Freeman et al 2009;Varadarajan et al 2011;Warren et al 2011), but can suffer from low efficiency and high levels of nonspecific amplification, contamination by short fragments from RNA degradation, or incomplete cDNA synthesis.…”

mentioning

confidence: 99%

Network properties derived from deep sequencing of human B-cell receptor repertoires delineate B-cell populations

et al. 2013

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The adaptive immune response selectively expands B-and T-cell clones following antigen recognition by B-and T-cell receptors (BCR and TCR), respectively. Next-generation sequencing is a powerful tool for dissecting the BCR and TCR populations at high resolution, but robust computational analyses are required to interpret such sequencing. Here, we develop a novel computational approach for BCR repertoire analysis using established next-generation sequencing methods coupled with network construction and population analysis. BCR sequences organize into networks based on sequence diversity, with differences in network connectivity clearly distinguishing between diverse repertoires of healthy individuals and clonally expanded repertoires from individuals with chronic lymphocytic leukemia (CLL) and other clonal blood disorders. Network population measures defined by the Gini Index and cluster sizes quantify the BCR clonality status and are robust to sampling and sequencing depths. BCR network analysis therefore allows the direct and quantifiable comparison of BCR repertoires between samples and intraindividual population changes between temporal or spatially separated samples and over the course of therapy.

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Epitope-Specific Human Influenza Antibody Repertoires Diversify by B Cell Intraclonal Sequence Divergence and Interclonal Convergence

Cited by 79 publications

References 42 publications

Focused antibody response to influenza linked to antigenic drift

Focused antibody response to influenza linked to antigenic drift

Genetic measurement of memory B-cell recall using antibody repertoire sequencing

Network properties derived from deep sequencing of human B-cell receptor repertoires delineate B-cell populations

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