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DNA中的双链断裂在体外会抑制核苷酸切除修复。

Double strand breaks in DNA inhibit nucleotide excision repair in vitro.

作者信息

Calsou P, Frit P, Salles B

机构信息

Institut de Pharmacologie et de Biologie Structurale, CNRS, UPR 9062, 205 route de Narbonne, 31077 Toulouse, France.

出版信息

J Biol Chem. 1996 Nov 1;271(44):27601-7. doi: 10.1074/jbc.271.44.27601.

Abstract

Nucleotide excision repair (NER) was measured in human cell extracts incubated with either supercoiled or linearized damaged plasmid DNA as repair substrate. NER, as quantified by the extent of repair synthesis activity, was reduced by up to 80% in the case of linearized plasmid DNA when compared with supercoiled DNA. An excess of undamaged linearized plasmid in the repair mixture did not interfere with DNA repair synthesis activity on a supercoiled damaged plasmid, indicating a cis-acting inhibiting effect. In contrast, gaps on circular or linearized plasmids were filled in identically by the DNA polymerases operating in the extracts. When the extent of damage-dependent incision activity was measured, a approximately 70% reduction of repair incision activity by human cell extract was observed on linearized damaged plasmids. Recessed, protruding, or blunt ends were similarly inhibitory. NER activity was partly restored when the extracts were preincubated with autoimmune human sera containing antibodies against the nuclear DNA end-binding heterodimer Ku. In addition, the inhibition of repair activity on linear damaged plasmids was released in extracts from rodent cells deficient in Ku activity but not in extracts from murine scid cells devoid of Ku-associated DNA-dependent kinase activity.

摘要

在以超螺旋或线性化损伤质粒DNA作为修复底物孵育的人细胞提取物中测定核苷酸切除修复(NER)。与超螺旋DNA相比,线性化质粒DNA情况下,通过修复合成活性程度定量的NER降低了多达80%。修复混合物中过量的未损伤线性化质粒不会干扰超螺旋损伤质粒上的DNA修复合成活性,表明存在顺式作用抑制效应。相反,提取物中起作用的DNA聚合酶对环状或线性化质粒上的缺口进行相同程度的填补。当测量损伤依赖性切口活性程度时,观察到在人细胞提取物中,线性化损伤质粒上的修复切口活性降低了约70%。凹陷、突出或平端同样具有抑制作用。当提取物与含有针对核DNA末端结合异二聚体Ku的抗体的自身免疫人血清预孵育时,NER活性部分恢复。此外,在缺乏Ku活性的啮齿动物细胞提取物中,线性损伤质粒上的修复活性抑制被解除,但在缺乏Ku相关DNA依赖性激酶活性的小鼠scid细胞提取物中未被解除。

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