Genetics and Breeding Unit, United States Meat Animal Research Center, ARS, USDA, Clay Center, NE, USA.
BMC Immunol. 2012 Sep 14;13:52. doi: 10.1186/1471-2172-13-52.
Vertebrate immune systems generate diverse repertoires of antibodies capable of mediating response to a variety of antigens. Next generation sequencing methods provide unique approaches to a number of immuno-based research areas including antibody discovery and engineering, disease surveillance, and host immune response to vaccines. In particular, single-molecule circular consensus sequencing permits the sequencing of antibody repertoires at previously unattainable depths of coverage and accuracy. We approached the bovine immunoglobulin G (IgG) repertoire with the objective of characterizing diversity of expressed IgG transcripts. Here we present single-molecule real-time sequencing data of expressed IgG heavy-chain repertoires of four individual cattle. We describe the diversity observed within antigen binding regions and visualize this diversity using a network-based approach.
We generated 49,945 high quality cDNA sequences, each spanning the entire IgG variable region from four Bos taurus calves. From these sequences we identified 49,521 antigen binding regions using the automated Paratome web server. Approximately 9% of all unique complementarity determining 2 (CDR2) sequences were of variable lengths. A bimodal distribution of unique CDR3 sequence lengths was observed, with common lengths of 5-6 and 21-25 amino acids. The average number of cysteine residues in CDR3s increased with CDR3 length and we observed that cysteine residues were centrally located in CDR3s. We identified 19 extremely long CDR3 sequences (up to 62 amino acids in length) within IgG transcripts. Network analyses revealed distinct patterns among the expressed IgG antigen binding repertoires of the examined individuals.
We utilized circular consensus sequencing technology to provide baseline data of the expressed bovine IgG repertoire that can be used for future studies important to livestock research. Somatic mutation resulting in base insertions and deletions in CDR2 further diversifies the bovine antibody repertoire. In contrast to previous studies, our data indicate that unusually long CDR3 sequences are not unique to IgM antibodies in cattle. Centrally located cysteine residues in bovine CDR3s provide further evidence that disulfide bond formation is likely of structural importance. We hypothesize that network or cluster-based analyses of expressed antibody repertoires from controlled challenge experiments will help identify novel natural antigen binding solutions to specific pathogens of interest.
脊椎动物的免疫系统产生了多样化的抗体库,能够介导对各种抗原的反应。下一代测序方法为许多基于免疫的研究领域提供了独特的方法,包括抗体发现和工程、疾病监测以及宿主对疫苗的免疫反应。特别是,单分子圆形共识测序允许以前无法达到的深度和准确性对抗体库进行测序。我们采用了牛免疫球蛋白 G(IgG)库,旨在描述表达 IgG 转录物的多样性。在这里,我们提出了四个个体牛的表达 IgG 重链库的单分子实时测序数据。我们描述了在抗原结合区域内观察到的多样性,并使用基于网络的方法可视化这种多样性。
我们生成了 49945 个高质量的 cDNA 序列,每个序列都跨越了来自 4 头 Bos taurus 小牛的整个 IgG 可变区。从这些序列中,我们使用自动 Paratome 网络服务器识别了 49521 个抗原结合区。所有独特的互补决定区 2(CDR2)序列中,约有 9%的序列长度可变。独特 CDR3 序列长度呈双峰分布,常见长度为 5-6 和 21-25 个氨基酸。CDR3 中的半胱氨酸残基数量随着 CDR3 长度的增加而增加,并且我们观察到半胱氨酸残基位于 CDR3 的中心。我们在 IgG 转录本中鉴定了 19 个非常长的 CDR3 序列(长度达 62 个氨基酸)。网络分析揭示了所检查个体的表达 IgG 抗原结合库之间的独特模式。
我们利用圆形共识测序技术为牛表达 IgG 库提供了基线数据,可用于对家畜研究很重要的未来研究。CDR2 中的体细胞突变导致碱基插入和缺失,进一步多样化了牛的抗体库。与之前的研究不同,我们的数据表明,在牛中,异常长的 CDR3 序列并非 IgM 抗体所特有。牛 CDR3 中中心位置的半胱氨酸残基进一步表明,二硫键的形成可能具有结构重要性。我们假设,对特定感兴趣病原体的受控挑战实验中表达抗体库的网络或聚类分析将有助于识别针对新型天然抗原结合解决方案。
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