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Correspondence between radioactive and functional methods in the quality control of DNA restriction and modifying enzymes.

作者信息

Trujillo L E, Pupo E, Miranda F, Pérez E, González E

机构信息

Molecular Biology Department, Center for Genetic Engineering and Biotechnology, (CIGB), Havana City, Cuba.

出版信息

Rev Latinoam Microbiol. 1996 Jan-Mar;38(1):31-7.

PMID:8783903
Abstract

We evaluated the use of two radiolabeled lambda DNA/Hpa II substrates to detect 5'-->3', 3'-->5' single and double stranded DNA dependent exonuclease and phosphatase activities found as contaminants in restriction and modifying enzyme preparations. Looking for the meaning of the radioactive assays results in a real cloning experience, we performed a cloning simulation assay using the same conditions established for the radioactive assay (enzyme units and pmols of DNA ends). As a result, we found that for degradation percentages of the radioactive DNA substrate per enzyme unit below 0.5, the false positives in the cloning stimulation assay were less than 5%. This conditions could ensure a good performance of the enzyme preparations for cloning experiments. Finally, we described the use of the radiolabeled [gamma 33P] ATP lambda Hpa II DNA substrate to detect 5'-->3' single stranded DNA dependent exonuclease and phosphatase contaminating activities in some critical steps of the purification process of the restriction enzyme Kpn I.

摘要

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