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Folding pathway for partially folded rabbit muscle creatine kinase

机译:部分折叠的兔肌肉肌酸激酶的折叠途径

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Rabbit muscle creatine kinase (CK) was modified by 5,5'-dithio-bis(2-nitrobenzoic acid) accompanied by 3 M guanidine hydrochloride denaturation to produce a partially folded state with modified thiol groups. The partially folded CK was in a monomeric state detected by size exclusion chromatography, native-polyacrylamide gel electrophoresis, circular dichroism, and intrinsic fluorescence studies. After dithiothreitol (DTT) treatment, about 70% CK activity was regained with a two-phase kinetic course. Rate constants calculated for regaining of activity and refolding were compared with those for CK modified with various treatments to show that refolding and recovery of activity were synchronized. To further characterize the partially folded CK state and its folding pathway, the molecular chaperone GroEL was used to evaluate whether it can bind with partly folded CK during refolding, and 1-anilinonaphthalene-8-sulfonate was used to detect the hydrophobic surface of the monomeric state of CK. The monomeric state of CK did not bind with GroEL, although it had a larger area of hydrophobic surface relative to the native state. These results may provide different evidence for the structural requirement of GroEL recognition to the substrate protein compared with previously reported results that GroEL bound with substrate proteins mainly through hydrophobic surface. The present study provides data for a monomeric intermediate trapped by the modification of the SH groups during the refolding of CK. Schemes are given for explaining both the partial folding CK pathway and the refolding pathway.
机译:通过5,5'-二硫代-双(2-硝基苯甲酸)修饰兔肌肉肌酸激酶(CK),伴随3 M盐酸胍变性,产生带有修饰硫醇基团的部分折叠状态。通过尺寸排阻色谱,天然聚丙烯酰胺凝胶电泳,圆二色性和固有荧光研究检测到部分折叠的CK处于单体状态。二硫苏糖醇(DTT)处理后,通过两阶段动力学过程恢复了约70%的CK活性。将为恢复活动和重新折叠而计算的速率常数与经各种处理修饰的CK的速率常数进行比较,以表明活动的重新折叠和恢复是同步的。为了进一步表征部分折叠的CK状态及其折叠途径,使用分子伴侣GroEL评估其在重折叠过程中是否可以与部分折叠的CK结合,并使用1-苯胺基萘-8-磺酸盐检测单体的疏水表面。 CK状态。 CK的单体态虽然与天然态相比具有更大的疏水表面面积,但并未与GroEL结合。与先前报道的结果GroEL主要通过疏水表面与底物蛋白结合的结果相比,这些结果可能为GroEL识别底物蛋白的结构要求提供了不同的证据。本研究提供了在CK的重折叠过程中被SH基团的修饰所捕获的单体中间体的数据。给出了用于解释部分折叠的CK途径和重折叠途径的方案。

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