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通过寡核苷酸杂交分离7号染色体上含有稀有切割酶识别位点的克隆。

Isolation of clones on chromosome 7 that contain recognition sites for rare-cutting enzymes by oligonucleotide hybridization.

作者信息

Melmer G, Sood R, Rommens J, Rego D, Tsui L C, Buchwald M

机构信息

Research Institute, Hospital for Sick Children, Toronto, Ontario, Canada.

出版信息

Genomics. 1990 Jun;7(2):173-81. doi: 10.1016/0888-7543(90)90538-6.

Abstract

Five G/C-containing oligonucleotides that include the recognition sequences of rare-cutting restriction enzymes have been used to isolate almost 100 different genomic segments from chromosome 7 that contain recognition sites for those enzymes. Hybridization and washing at 27 degrees C allow the use of 8-bp radiolabeled oligonucleotides to detect specific G/C-containing sequences in less than 1 ng of cloned DNA. This method was used to isolate 9 positive clones from 138 previously isolated single-copy probes from a flow-sorted chromosome 7 library. The specificity of the method was confirmed by showing that clones that gave positive hybridization signals also contained the corresponding restriction site. The oligonucleotides were also used to analyze approximately 12,000 kb of genomic sequence from a newly constructed chromosome 7 cosmid library that yielded 88 positive cosmids from 350 analyzed. The average distances between binding sites ranged from 200 to 690 kb and was independent of the number of CpG residues present in the oligonucleotide. Confirmation that clones containing restriction sites for these rare-cutting enzymes are located near genes was obtained by hybridization to RNA and cross-species DNA blots.

摘要

五个含G/C的寡核苷酸,其中包含稀有切割限制酶的识别序列,已被用于从7号染色体中分离出近100个不同的基因组片段,这些片段含有那些酶的识别位点。在27摄氏度下进行杂交和洗涤,使得能够使用8碱基对放射性标记的寡核苷酸,在不到1纳克的克隆DNA中检测特定的含G/C序列。该方法用于从一个经流式分选的7号染色体文库中,从138个先前分离的单拷贝探针中分离出9个阳性克隆。通过显示给出阳性杂交信号的克隆也包含相应的限制酶切位点,证实了该方法的特异性。这些寡核苷酸还用于分析一个新构建的7号染色体黏粒文库中约12,000 kb的基因组序列,在分析的350个黏粒中产生了88个阳性黏粒。结合位点之间的平均距离在200至690 kb之间,且与寡核苷酸中存在的CpG残基数量无关。通过与RNA和跨物种DNA印迹杂交,证实了含有这些稀有切割酶限制位点的克隆位于基因附近。

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