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在单体rop中构建血红素结合位点。

Engineering heme binding sites in monomeric rop.

作者信息

Di Nardo Giovanna, Di Venere Almerinda, Mei Giampiero, Sadeghi Sheila J, Wilson Jon R, Gilardi Gianfranco

机构信息

Department of Human and Animal Biology, University of Turin, Turin, Italy.

出版信息

J Biol Inorg Chem. 2009 May;14(4):497-505. doi: 10.1007/s00775-009-0465-0. Epub 2009 Jan 17.

Abstract

Heme ligands were introduced in the hydrophobic core of an engineered monomeric ColE1 repressor of primer (rop-S55) in two different layers of the heptad repeat. Mutants rop-L63M/F121H (layer 1) and rop-L56H/L113H (layer 3) were found to bind heme with a K (D) of 1.1 +/- 0.2 and 0.47 +/- 0.07 microM, respectively. The unfolding of heme-bound and heme-free mutants, in the presence of guanidinium hydrochloride, was monitored by both circular dichroism and fluorescence spectroscopy. For the heme-bound rop mutants, the total free energy change was 0.5 kcal/mol higher in the layer 3 mutant compared with that in the layer1 mutant. Heme binding also stabilized these mutants by increasing the [DGobsH2O] by 1.4 and 1.8 kcal/mol in rop-L63M/F121H and rop-L56H/L113H, respectively. The reduction potentials measured by spectroelectrochemical titrations were calculated to be -154 +/- 2 mV for rop-56H/113H and -87.5 +/- 1.2 mV for rop-L63M/F121H. The mutant designed to bind heme in a more buried environment (layer 3) showed tighter heme binding, a higher stability, and a different reduction potential compared with the mutant designed to bind heme in layer 1.

摘要

血红素配体被引入到引物(rop-S55)的工程化单体ColE1阻遏物的疏水核心中,位于七肽重复序列的两个不同层。发现突变体rop-L63M/F121H(第1层)和rop-L56H/L113H(第3层)分别以1.1±0.2和0.47±0.07微摩尔的解离常数(KD)结合血红素。在盐酸胍存在下,通过圆二色性和荧光光谱监测血红素结合型和无血红素突变体的解折叠。对于血红素结合型rop突变体,第3层突变体的总自由能变化比第1层突变体高0.5千卡/摩尔。血红素结合还通过分别使rop-L63M/F121H和rop-L56H/L113H的[DGobsH2O]增加1.4和1.8千卡/摩尔来稳定这些突变体。通过光谱电化学滴定测量的还原电位经计算,rop-56H/113H为-154±2毫伏,rop-L63M/F121H为-87.5±1.2毫伏。与设计用于在第1层结合血红素的突变体相比,设计用于在更隐蔽环境(第3层)中结合血红素的突变体显示出更紧密的血红素结合、更高的稳定性和不同的还原电位。

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