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利用单色氨酸突变体对色氨酸阻遏物进行荧光猝灭研究。

Fluorescence quenching studies of Trp repressor using single-tryptophan mutants.

作者信息

Blicharska Z, Wasylewski Z

机构信息

Department of Physical Biochemistry, Jagellonian University, Kraków, Poland.

出版信息

J Protein Chem. 1995 Nov;14(8):739-46. doi: 10.1007/BF01886913.

Abstract

Time-resolved and steady-state fluorescence have been used to resolve the heterogeneous emission of single-tryptophan-containing mutants of Trp repressors W19F and W99F into components. Using iodide as the quencher, the fluorescence-quenching-resolved spectra (FQRS) have been obtained The FQRS method shows that the fluorescence emission of Trp99 can be resolved into two component spectra characterized by maxima of fluorescence emission at 338 and 328 nm. The redder component is exposed to the solvent and participates in about 21% of the total fluorescence emission of TrpR W19F. The second component is inacessible to iodide, but is quenched by acrylamide. The tryptophan residue 19 present in TrpR W99F can be resolved into two component spectra using the FQRS method and iodide as a quencher. Both components of Trp19 exhibit similar maxima of emission at 322-324 nm and both are quenchable by iodide. The component more quenchable by iodide participates in about 38% of the total TrpR W99F emission. The fluorescence lifetime measurements as a function of iodide concentration support the existence of two classes of Trp99 and Trp19 in the Trp repressor. Our results suggest that the Trp aporepressor can exist in the ground state in two distinct conformational states which differ in the microenvironment of the Trp residues.

摘要

时间分辨荧光和稳态荧光已被用于将色氨酸阻遏物W19F和W99F的含单个色氨酸突变体的非均匀发射解析为不同组分。以碘化物作为猝灭剂,获得了荧光猝灭分辨光谱(FQRS)。FQRS方法表明,Trp99的荧光发射可解析为两个组分光谱,其特征在于荧光发射最大值分别在338和328 nm处。波长较长的组分暴露于溶剂中,占TrpR W19F总荧光发射的约21%。第二个组分碘化物无法接近,但可被丙烯酰胺猝灭。使用FQRS方法并以碘化物作为猝灭剂,TrpR W99F中存在的色氨酸残基19可解析为两个组分光谱。Trp19的两个组分在322 - 324 nm处均表现出相似的发射最大值,且均可被碘化物猝灭。被碘化物猝灭程度更高的组分占TrpR W99F总发射的约38%。作为碘化物浓度函数的荧光寿命测量结果支持色氨酸阻遏物中存在两类Trp99和Trp19。我们的结果表明,色氨酸无辅阻遏物可以以两种不同的构象状态存在于基态,这两种状态在色氨酸残基的微环境上有所不同。

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