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Structure of an archaeal PCNA1-PCNA2-FEN1 complex: elucidating PCNA subunit and client enzyme specificity

机译:古细菌PCNA1-PCNA2-FEN1复合物的结构:阐明PCNA亚基和客户酶的特异性

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The archaeal/eukaryotic proliferating cell nuclear antigen (PCNA) toroidal clamp interacts with a host of DNA modifying enzymes, providing a stable anchorage and enhancing their respective processivities. Given the broad range of enzymes with which PCNA has been shown to interact, relatively little is known about the mode of assembly of functionally meaningful combinations of enzymes on the PCNA clamp. We have determined the X-ray crystal structure of the Sulfolobus solfataricus PCNA1-PCNA2 heterodimer, bound to a single copy of the flap endonuclease FEN1 at 2.9 angstrom resolution. We demonstrate the specificity of interaction of the PCNA subunits to form the PCNA1-PCNA2-PCNA3 heterotrimer, as well as providing a rationale for the specific interaction of the C-terminal PIP-box motif of FEN1 for the PCNA1 subunit. The structure explains the specificity of the individual archaeal PCNA subunits for selected repair enzyme 'clients', and provides insights into the co-ordinated assembly of sequential enzymatic steps in PCNA-scaffolded DNA repair cascades.
机译:古细菌/真核生物增殖细胞核抗原(PCNA)环形夹具与许多DNA修饰酶相互作用,提供稳定的锚定并增强它们各自的加工能力。鉴于已显示PCNA与之相互作用的酶种类繁多,对PCNA钳上酶的功能上有意义的组合的组装模式知之甚少。我们已经确定了Sulfolobus solfataricus PCNA1-PCNA2异二聚体的X射线晶体结构,其以2.9埃的分辨率与襟翼内切核酸酶FEN1的单个副本结合。我们证明了PCNA亚基形成PCNA1-PCNA2-PCNA3异源三聚体相互作用的特异性,以及为PCNA1亚基的FEN1的C末端PIP盒基序的特定相互作用提供了理论基础。该结构解释了单个古细菌PCNA亚基对所选修复酶“客户”的特异性,并提供了对PCNA骨架DNA修复级联反应中顺序酶促步骤的协调组装的见解。

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