[laidlawii PG-8中DNA依赖性DNA聚合酶的色谱性质]。

Mikrobiologicheskii zhurnal Pub Date : 1992-01-01
S V Bezuglyĭ, I G Skripal', V V Babichev
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引用次数: 0

摘要

从laidlawii PG-8中分离出DNA依赖性DNA聚合酶(未被deae纤维素吸附在色谱柱上的DNA聚合酶I和被该色谱柱吸附并被0.3 M NaCl洗脱的DNA聚合酶II)。经肝素-sepharose (0.35 M NaCl洗脱)和聚u -sepharose (0.3 M NaCl洗脱)分步处理,得到均相的dna -聚合酶I。在电泳图上以一个分子量为72 kDalton的多肽表示。在肝素-sepharose (0.3 M NaCl洗脱)和聚- a -sepharose (0.25 M NaCl洗脱)上依次处理,也得到了均相的第二种形式的DNA聚合酶:表现出聚合酶活性的蛋白是分子量为45 kDalton的多肽。
本文章由计算机程序翻译,如有差异,请以英文原文为准。
[The chromatographic properties of the DNA-dependent DNA polymerases from Acholeplasma laidlawii PG-8].

The DNA-dependent DNA-polymerase (DNA polymerase I which is not sorbed on the column with DEAE-cellulose, and DNA-polymerase II, which is absorbed by this column and is eluted from it by 0.3 M of NaCl), have been isolated from Acholeplasma laidlawii PG-8. DNA-polymerase I in homogeneous state was obtained as a result of the stepwise treatment by heparin-sepharose (elution at 0.35 M of NaCl) and poly-U-sepharose (elution at 0.3 M of NaCl). It was presented on the electrophoregram by one polypeptide with molecular weight of 72 kDalton. The second form of DNA polymerase was also obtained in homogeneous state as a result of sequential treatment on heparin-sepharose (elution at 0.3 M of NaCl) and on poly-A-sepharose (elution at 0.25 M of NaCl): the protein which had manifested polymerase activity was a polypeptide with molecular weight of 45 kDalton.

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