Specific amplification by PCR of rearranged genomic variable regions of immunoglobulin genes from mouse hybridoma cells.

J Berdoz, T P Monath, J P Kraehenbuhl
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引用次数: 10

Abstract

We have designed a novel strategy for the isolation of the rearranged genomic fragments encoding the L-VH-D-JH and L-V kappa/lambda-J kappa/lambda regions of mouse immunoglobulin genes. This strategy is based on the PCR amplification of genomic DNA from mouse hybridomas using multiple specific primers chosen in the 5'-untranslated region and in the intron downstream of the rearranged JH/J kappa/lambda sequences. Variable regions with intact coding sequences, including full-length leader peptides (L) can be obtained without previous DNA sequencing. Our strategy is based on a genomic template that produces fragments that do not need to be adapted for recombinant antibody expression, thus facilitating the generation of chimeric and isotype-switched immunoglobulins.

小鼠杂交瘤细胞免疫球蛋白基因基因组可变区重排的PCR特异性扩增。
我们设计了一种新的策略来分离编码小鼠免疫球蛋白基因的L-VH-D-JH和L-V kappa/lambda- j kappa/lambda区域的重排基因组片段。该策略基于对小鼠杂交瘤基因组DNA的PCR扩增,使用在重排的JH/J kappa/lambda序列的5'-未翻译区和内含子下游选择的多个特异性引物。具有完整编码序列的可变区域,包括全长先导肽(L),无需先前的DNA测序即可获得。我们的策略是基于基因组模板,该模板产生的片段不需要适应重组抗体表达,从而促进嵌合和同型转换免疫球蛋白的产生。
本文章由计算机程序翻译,如有差异,请以英文原文为准。
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