首页> 外文OA文献 >Use of synthetic oligonucleotide probes complementary to genes for human HLA-DR alpha and beta as extension primers for the isolation of 5'-specific genomic clones.
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Use of synthetic oligonucleotide probes complementary to genes for human HLA-DR alpha and beta as extension primers for the isolation of 5'-specific genomic clones.

机译:与人类HLA-DRα和β基因互补的合成寡核苷酸探针作为扩展引物用于分离5'-特异性基因组克隆。

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摘要

We have synthesized 175-nucleotide-long probes for the DNA of human histocompatibility antigens HLA-DR alpha and beta by extending on poly(A)+ mRNA from B-cell lines with short synthetic deoxyribonucleotide primers complementary to the predicted nucleotide sequence of the NH2 terminus of both polypeptides. The synthesis of the probe for the alpha-chain DNA was a two-step process starting with 11-mers which were extended by dideoxynucleotide chain termination experiments to a 20-mer of predicted sequence. The synthesized 20-mer was then used to generate a 175-nucleotide cDNA probe which was shown to encode the appropriate amino acids for the alpha chain and was used to select a human genomic DNA clone containing the coding sequences for HLA-DR alpha. For the beta polypeptide an 18-mer homologous to the NH2-terminal sequence of a cDNA clone from another B-cell line was used to extend on poly(A)+ mRNA isolated from a B-cell line. Preliminary sequence analysis of a 175-base-long extension product indicates a match of the cDNA sequence to the published sequence of a clone for HLA-DR beta. Information from these extension experiments helps to establish the sensitivity and specificity of the primer extension method.
机译:我们已经用人合成相容性抗原HLA-DR alpha和beta的DNA合成了175个核苷酸长的探针,方法是用短合成脱氧核糖核苷酸引物(与NH2的预期核苷酸序列互补)在B细胞系的poly(A)+ mRNA上延伸两种多肽的末端。 α链DNA探针的合成是一个两步过程,从11聚体开始,通过双脱氧核苷酸链终止实验将其扩展到20聚体的预测序列。然后,将合成的20-mer用于产生175个核苷酸的cDNA探针,该探针显示为编码α链的合适氨基酸,并用于选择包含HLA-DRα编码序列的人基因组DNA克隆。对于β多肽,与来自另一个B细胞系的cDNA克隆的NH 2末端序列同源的18聚体用于在从B细胞系分离的poly(A)+ mRNA上延伸。对175个碱基长的延伸产物的初步序列分析表明cDNA序列与HLA-DR beta克隆的已公开序列匹配。这些延伸实验的信息有助于确定引物延伸方法的敏感性和特异性。

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