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肌酸激酶 B 的亚膜募集支持巨噬细胞中动态肌动蛋白基突起的形成,并依赖于其 C 端柔性环。

Submembranous recruitment of creatine kinase B supports formation of dynamic actin-based protrusions of macrophages and relies on its C-terminal flexible loop.

机构信息

Department of Cell Biology, Radboud Institute for Molecular Life Sciences, Radboud University Medical Centre, PO Box 9101, 6500 HB, Nijmegen, The Netherlands.

Centre for Molecular and Biomolecular Informatics, Radboud Institute for Molecular Life Sciences, Radboud University Medical Centre, PO Box 9101, 6500 HB, Nijmegen, The Netherlands.

出版信息

Eur J Cell Biol. 2015 Feb;94(2):114-27. doi: 10.1016/j.ejcb.2014.11.002. Epub 2014 Nov 24.

DOI:10.1016/j.ejcb.2014.11.002
PMID:25538032
Abstract

Subcellular partitioning of creatine kinase contributes to the formation of patterns in intracellular ATP distribution and the fuelling of cellular processes with a high and sudden energy demand. We have previously shown that brain-type creatine kinase (CK-B) accumulates at the phagocytic cup in macrophages where it is involved in the compartmentalized generation of ATP for actin remodeling. Here, we report that CK-B catalytic activity also helps in the formation of protrusive ruffle structures which are actin-dependent and abundant on the surface of both unstimulated and LPS-activated macrophages. Recruitment of CK-B to these structures occurred transiently and inhibition of the enzyme's catalytic activity with cyclocreatine led to a general smoothening of surface morphology as visualized by scanning electron microscopy. Comparison of the dynamics of distribution of YFP-tagged CK-mutants and isoforms by live imaging revealed that amino acid residues in the C-terminal segment (aa positions 323-330) that forms one of the protein's two mobile loops are involved in partitioning over inner regions of the cytosol and nearby sites where membrane protrusions occur during induction of phagocytic cup formation. Although wt CK-B, muscle-type CK (CK-M), and a catalytically dead CK-B-E232Q mutant with intact loop region were normally recruited from the cytosolic pool, no dynamic transition to the phagocytic cup area was seen for the CK-homologue arginine kinase and a CK-B-D326A mutant protein. Bioinformatics analysis helped us to predict that conformational flexibility of the C-terminal loop, independent of conformational changes induced by substrate binding or catalytic activity, is likely involved in exposing the enzyme for binding at or near the sites of membrane protrusion formation.

摘要

肌酸激酶的亚细胞分区有助于形成细胞内 ATP 分布的模式,并为具有高能量需求的细胞过程提供燃料。我们之前已经表明,脑型肌酸激酶(CK-B)在巨噬细胞的吞噬杯中积累,在吞噬杯中它参与了肌动蛋白重塑的局部 ATP 生成。在这里,我们报告说 CK-B 的催化活性还有助于形成突起皱褶结构,这些结构是肌动蛋白依赖性的,并且在未刺激和 LPS 激活的巨噬细胞表面都很丰富。CK-B 向这些结构的募集是短暂的,用环肌酸抑制酶的催化活性会导致扫描电子显微镜观察到的表面形态普遍变平。通过活细胞成像比较 YFP 标记的 CK 突变体和同工型的分布动力学表明,形成蛋白质两个可移动环之一的 C 末端片段(aa 位置 323-330)中的氨基酸残基参与了细胞质内部区域的分区以及在诱导吞噬杯形成期间发生的膜突起附近的位点。虽然 wt CK-B、肌型 CK(CK-M)和具有完整环区的催化失活 CK-B-E232Q 突变体通常从细胞质池中招募,但 CK 同源物精氨酸激酶和 CK-B-D326A 突变体蛋白没有向吞噬杯区域进行动态转变。生物信息学分析帮助我们预测,C 末端环的构象灵活性,独立于底物结合或催化活性引起的构象变化,可能涉及到暴露酶以在膜突起形成的部位或附近进行结合。

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