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细菌磷酸苏氨酸裂解酶对苏氨酸的消除化作用会迅速导致活细胞中有丝分裂原激活蛋白激酶(MAPK)发生交联。

Threonine eliminylation by bacterial phosphothreonine lyases rapidly causes cross-linking of mitogen-activated protein kinase (MAPK) in live cells.

作者信息

Meijer Benoit M, Jang Suk Min, Guerrera Ida C, Chhuon Cerina, Lipecka Joanna, Reisacher Caroline, Baleux Françoise, Sansonetti Philippe J, Muchardt Christian, Arbibe Laurence

机构信息

From the Team genomic plasticity and infection, Department of Immunology, Infectiology and Hematology, Institut Necker Enfants Malades, INSERM U1151, CNRS UMR 8253, 75993 Paris CEDEX 14, France.

the Université Paris Diderot, Sorbonne Paris Cité, Cellule Pasteur UPMC, 75724 Paris, France.

出版信息

J Biol Chem. 2017 May 12;292(19):7784-7794. doi: 10.1074/jbc.M117.775940. Epub 2017 Mar 21.

Abstract

Old long-lived proteins contain dehydroalanine (Dha) and dehydrobutyrine (Dhb), two amino acids engendered by dehydration of serines and threonines, respectively. Although these residues have a suspected role in protein cross-linking and aggregation, their direct implication has yet to be determined. Here, we have taken advantage of the ability of the enteropathogen to convert the phosphothreonine residue of the pT--pY consensus sequence of ERK and p38 into Dhb and followed the impact of dehydration on the fate of the two MAPKs. To that end, we have generated the first antibodies recognizing Dhb-modified proteins and allowing tracing them as they form. We showed that Dhb modifications accumulate in a long-lasting manner -infected cells, causing subsequent formation of covalent cross-links of MAPKs. Moreover, the Dhb signal correlates precisely with the activation of the type III secretion apparatus, thus evidencing injectisome activity. This observation is the first to document a causal link between Dhb formation and protein cross-linking in live cells. Detection of eliminylation is a new avenue to phosphoproteome regulation in eukaryotes that will be instrumental for the development of type III secretion inhibitors.

摘要

老化的长寿蛋白含有脱氢丙氨酸(Dha)和脱氢丁氨酸(Dhb),这两种氨基酸分别由丝氨酸和苏氨酸脱水形成。尽管这些残基在蛋白质交联和聚集方面可能发挥作用,但其直接影响尚未确定。在这里,我们利用肠道病原体的能力,将ERK和p38的pT-pY共有序列中的磷酸苏氨酸残基转化为Dhb,并追踪脱水对这两种丝裂原活化蛋白激酶(MAPK)命运的影响。为此,我们制备了首批识别Dhb修饰蛋白并能在其形成过程中对其进行追踪的抗体。我们发现,Dhb修饰在感染细胞中以持久的方式积累,导致随后MAPK共价交联的形成。此外,Dhb信号与III型分泌装置的激活精确相关,从而证明了注射体的活性。这一观察结果首次证明了活细胞中Dhb形成与蛋白质交联之间的因果关系。消除磷酸化的检测是真核生物磷酸蛋白质组调控的一条新途径,将有助于III型分泌抑制剂的开发。

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