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使用位点特异性13C标记的泛醌-10对球形红杆菌R26光合反应中心中功能不对称的QA结合进行13C魔角旋转核磁共振表征。

13C magic angle spinning NMR characterization of the functionally asymmetric QA binding in Rhodobacter sphaeroides R26 photosynthetic reaction centers using site-specific 13C-labeled ubiquinone-10.

作者信息

van Liemt W B, Boender G J, Gast P, Hoff A J, Lugtenburg J, de Groot H J

机构信息

Leiden Institute of Chemistry, Gorlaeus Laboratories, The Netherlands.

出版信息

Biochemistry. 1995 Aug 15;34(32):10229-36. doi: 10.1021/bi00032a017.

Abstract

Photosynthetic reaction centers (RCs) of Rhodobacter sphaeroides R26 were reconstituted at the QA site with ubiquinone-10, selectively 13C-enriched on positions 1, 2, 3, 4, and 3-Me (IUPAC numbering). RCs dispersed in LDAO detergent were studied with 13C CP/MAS NMR spectroscopy at temperatures between 180 and 240 K, while RCs precipitated by removal of the detergent were investigated at ambient temperature and at temperatures down to 180 K. Electrostatic charge differences in QA induced by polarization from the protein are less than 0.02 electronic equivalent for any of the labeled positions. This includes the 4-carbonyl, which is therefore not significantly polarized by an electrostatic binding interaction with the protein. The QA site is slightly heterogeneous on the scale of the NMR as the observed line widths of the labels are between 150 and 300 Hz and inhomogeneous broadening is observed for the signals of positions 1, 2, and 3 upon cooling. This contrasts with earlier MAS observations for labels in the vicinity of the special pair. The chemical shifts are 184, 144, and 137 ppm for the labels at positions 1, 2, 3, and 12 ppm for the 3-methyl 13C. For the 4-carbonyl only at sample temperatures below approximately 255 K a CP/MAS response can be observed at 183 ppm. The principal components of the chemical shift tensors for the ring labels in QA were estimated using difference spectroscopy.(ABSTRACT TRUNCATED AT 250 WORDS)

摘要

球形红细菌R26的光合反应中心(RCs)在QA位点用10-泛醌重构,10-泛醌在1、2、3、4和3-甲基(IUPAC编号)位置选择性地富集13C。分散在LDAO去污剂中的RCs在180至240K的温度下用13C CP/MAS NMR光谱进行研究,而通过去除去污剂沉淀的RCs在室温及低至180K的温度下进行研究。对于任何标记位置,由蛋白质极化引起的QA中的静电荷差异小于0.02电子当量。这包括4-羰基,因此它不会因与蛋白质的静电结合相互作用而发生明显极化。在NMR尺度上,QA位点略有不均匀,因为观察到的标记线宽在150至300Hz之间,并且在冷却时观察到位置1、2和3的信号存在非均匀展宽。这与早期对特殊对附近标记的MAS观察结果形成对比。位置1、2、3处标记的化学位移为184、144和137ppm,3-甲基13C的化学位移为12ppm。仅对于4-羰基,在样品温度低于约255K时,在183ppm处可观察到CP/MAS响应。使用差示光谱法估计了QA中环标记的化学位移张量的主成分。(摘要截断于250字)

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