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通过锚定PCR-ELISA分析免疫球蛋白VH基因库。

Analysis of immunoglobulin VH gene repertoire by an anchored PCR-ELISA.

作者信息

Rassenti L Z, Kohsaka H, Kipps T J

机构信息

Sam & Rose Stein Institute for Research on Aging, University of California, San Diego, La Jolla 92093, USA.

出版信息

Ann N Y Acad Sci. 1995 Sep 29;764:463-73. doi: 10.1111/j.1749-6632.1995.tb55866.x.

DOI:10.1111/j.1749-6632.1995.tb55866.x
PMID:7486567
Abstract

We developed a novel technique to analyze the relative concentration of the expressed immunoglobulin (Ig) VH genes using an enzyme-linked immunosorbent assay (ELISA). Expressed Ig cDNA are amplified via anchored PCR and then subjected to a "nested PCR" reaction that attaches biotin to the 5' end of the antisense strand. This allows us to tether the antisense strand of PCR products onto avidin-coated ELISA plates. Digoxigenin-labeled oligonucleotides specific for the leader sequence sense strand of each major Ig VH gene subgroup are used to probe the plate-tethered, alkaline-denatured, and single-stranded antisense cDNA. Bound probes then are detected with alkaline-phosphatase-conjugated anti-digoxigenin antibodies. Using this method, we assessed the distribution of Ig VH genes used by IgM-expressing blood B cells of normal adults. We found the predominant subgroup is VH3, representing approximately half (range 41-59%) of the expressed IgM repertoire. The next largest subgroups used are VH4 (19-23%), VH1 (15-17%), and VH5 (7-11%). The VH2, VH6, and VH7 subgroups each constitute less than 3% of the expressed IgM repertoire. These results agree with those obtained using traditional and more laborious methods that analyze the distribution of Ig clones in cDNA libraries. In addition, we find that this method compares favorably in sensitivity and specificity to more conventional techniques for assessing the clonality of blood or tissue B-cell populations. This rapid and nonradioactive method should have utility for assessing the Ig repertoires expressed by normal, autoimmune, or neoplastic B-cell populations.

摘要

我们开发了一种新技术,利用酶联免疫吸附测定(ELISA)来分析表达的免疫球蛋白(Ig)VH基因的相对浓度。通过锚定PCR扩增表达的Ig cDNA,然后进行“巢式PCR”反应,将生物素连接到反义链的5'端。这使我们能够将PCR产物的反义链系在抗生物素蛋白包被的ELISA板上。使用针对每个主要Ig VH基因亚组的前导序列有义链的地高辛配体标记的寡核苷酸来探测固定在板上、经碱变性的单链反义cDNA。然后用碱性磷酸酶偶联的抗地高辛配体抗体检测结合的探针。使用这种方法,我们评估了正常成年人表达IgM的血液B细胞所使用的Ig VH基因的分布。我们发现主要亚组是VH3,约占表达的IgM库的一半(范围为41 - 59%)。其次使用最多的亚组是VH4(19 - 23%)、VH1(15 - 17%)和VH5(7 - 11%)。VH2、VH6和VH7亚组在表达的IgM库中各占不到3%。这些结果与使用传统且更费力的方法分析cDNA文库中Ig克隆分布所获得的结果一致。此外,我们发现该方法在灵敏度和特异性方面优于评估血液或组织B细胞群体克隆性的更传统技术。这种快速且无放射性的方法在评估正常、自身免疫或肿瘤性B细胞群体表达的Ig库方面应具有实用性。

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