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Isolation and characterization of mouse Xrcc-1, a DNA repair gene affecting ligation.

作者信息

Brookman K W, Tebbs R S, Allen S A, Tucker J D, Swiger R R, Lamerdin J E, Carrano A V, Thompson L H

机构信息

Biology and Biotechnology Research Program, Lawrence Livermore National Laboratory, Livermore, California 94551-0808.

出版信息

Genomics. 1994 Jul 1;22(1):180-8. doi: 10.1006/geno.1994.1359.

Abstract

Human DNA repair gene XRCC1 complements the strand-break rejoining defect in Chinese hamster mutant EM9 and encodes a protein that is apparently required for optimal activity of DNA ligase III. Toward the goal of producing transgenic mice that carry a mutation in the Xrcc-1 locus, the murine homolog of XRCC1 was cloned from both cosmid genomic and cDNA libraries. Upon transfection into EM9 cells, cosmids containing the functional mouse gene efficiently corrected (94-100%) the high sister-chromatid-exchange defect. Mouse Xrcc-1 is 26 kb in length, contains 17 exons, and maps by metaphase in situ hybridization to the 7A3-7B2 region of mouse chromosome 7. Isolated cDNA clones were highly truncated and were extended by anchored polymerase chain reactions. The 1893-bp open reading frame of mouse Xrcc-1 encodes 631 amino acids, compared with 633 for the human homolog. The predicted mouse Xrcc-1 protein of 69.1 kDa and pI of 5.95 is 86% identical and 93% similar to human XRCC1.

摘要

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