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开放阅读框克隆:开放阅读框DNA的鉴定、克隆及表达

Open reading frame cloning: identification, cloning, and expression of open reading frame DNA.

作者信息

Gray M R, Colot H V, Guarente L, Rosbash M

出版信息

Proc Natl Acad Sci U S A. 1982 Nov;79(21):6598-602. doi: 10.1073/pnas.79.21.6598.

Abstract

A plasmid was constructed that facilitates the cloning and expression of open reading frame DNA. A DNA fragment containing a bacterial promoter and the amino terminus of the cI gene of bacteriophage lambda was fused to an amino-terminally deleted version of the lacZ gene. An appropriate cloning site was inserted between these two fragments such that a frameshift mutation was introduced upstream of the lacZ-encoding DNA. This cloning vehicle produces a relatively low level of beta-galactosidase activity when introduced into Escherichia coli. The insertion of foreign DNA at the cloning site can reverse the frameshift mutation and generate plasmids that produce a relatively high level of beta-galactosidase activity. A large fraction of these plasmids produce a fusion protein that has a portion of the lambda cI protein at the amino terminus, the foreign protein segment in the middle, and the lacZ polypeptide at the carboxyl terminus. The production of a high level of beta-galactosidase and a large fusion polypeptide guarantees the cloning of a DNA fragment with at least one open reading frame that traverses the entirety of the fragment. Hence, the method can identify, clone, and express (as part of a larger fusion polypeptide) open reading frame DNA from among a large collection of DNA fragments.

摘要

构建了一种质粒,它有助于开放阅读框DNA的克隆和表达。将一个包含细菌启动子和噬菌体λ cI基因氨基末端的DNA片段与lacZ基因氨基末端缺失的版本融合。在这两个片段之间插入一个合适的克隆位点,使得在lacZ编码DNA的上游引入移码突变。当将这种克隆载体导入大肠杆菌时,它会产生相对较低水平的β-半乳糖苷酶活性。在克隆位点插入外源DNA可以逆转移码突变,并产生能产生相对较高水平β-半乳糖苷酶活性的质粒。这些质粒中的很大一部分会产生一种融合蛋白,该融合蛋白在氨基末端有一部分λ cI蛋白,中间是外源蛋白片段,羧基末端是lacZ多肽。高水平的β-半乳糖苷酶和大的融合多肽的产生保证了至少含有一个贯穿整个片段的开放阅读框的DNA片段的克隆。因此,该方法可以从大量DNA片段中鉴定、克隆并表达(作为更大融合多肽的一部分)开放阅读框DNA。

https://cdn.ncbi.nlm.nih.gov/pmc/blobs/3a2d/347175/d7ac159c99e5/pnas00460-0194-a.jpg

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