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Spo0F反应调节因子的丙氨酸突变体改变了芽孢形成起始中传感器激酶的特异性。

Alanine mutants of the Spo0F response regulator modifying specificity for sensor kinases in sporulation initiation.

作者信息

Jiang M, Tzeng Y L, Feher V A, Perego M, Hoch J A

机构信息

Division of Cellular Biology, Department of Molecular and Experimental Medicine, NX-1, The Scripps Research Institute, 10550 North Torrey Pines Road, La Jolla, CA 92037, USA.

出版信息

Mol Microbiol. 1999 Jul;33(2):389-95. doi: 10.1046/j.1365-2958.1999.01481.x.

DOI:10.1046/j.1365-2958.1999.01481.x
PMID:10411754
Abstract

Five single alanine substitution mutations in the Spo0F response regulator gave rise to mutant strains of Bacillus subtilis with seemingly normal sporulation that nevertheless rapidly segregated variants blocked in sporulation. The basis for this deregulated phenotype was postulated to be increased phosphorylation of the Spo0A transcription factor, resulting from enhanced phosphate input or decreased dephosphorylation of the phosphorelay. Strains bearing two of these Spo0F mutant proteins, Y13A and I17A, retained a requirement for KinA and KinB kinases in sporulation, whereas the remaining three, L66A, I90A and H101A, gave strains that sporulated well in the absence of both KinA and KinB. Sporulation of strains bearing L66A and H101A mutations was decreased in a mutant lacking KinA, KinB and KinC, but the strain bearing the I90A mutation required the further deletion of KinD to lower its sporulation frequency. The affected residues, L-66, I-90 and H-101, are involved in crucial hydrophobic contacts stabilizing the orientation of helix alpha4 of Spo0F. The data are consistent with the notion that these three mutations alter the conformation of the beta4-alpha4 loop of Spo0F that is known to contain residues critical for KinA:Spo0F recognition. As this loop has a propensity for multiple conformations, the spatial arrangement of this loop may play a critical role in kinase selection by Spo0F and might be altered by regulatory molecules interacting with Spo0F.

摘要

芽孢形成反应调节因子Spo0F中的五个单丙氨酸取代突变产生了枯草芽孢杆菌的突变菌株,这些菌株看似具有正常的芽孢形成能力,但仍会迅速分离出芽孢形成受阻的变体。这种失调表型的基础被推测是Spo0A转录因子的磷酸化增加,这是由于磷酸输入增强或磷酸传递的去磷酸化减少所致。携带这两种Spo0F突变蛋白Y13A和I17A的菌株在芽孢形成过程中仍需要KinA和KinB激酶,而其余三种L66A、I90A和H101A则使菌株在没有KinA和KinB的情况下也能良好地形成芽孢。携带L66A和H101A突变的菌株在缺乏KinA、KinB和KinC的突变体中芽孢形成减少,但携带I90A突变的菌株需要进一步缺失KinD才能降低其芽孢形成频率。受影响的残基L-66、I-90和H-101参与了稳定Spo0F的α4螺旋方向的关键疏水接触。这些数据与以下观点一致,即这三个突变改变了Spo0F的β4-α4环的构象,已知该环包含对KinA:Spo0F识别至关重要的残基。由于这个环具有多种构象的倾向,这个环的空间排列可能在Spo0F对激酶的选择中起关键作用,并且可能会被与Spo0F相互作用的调节分子改变。

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