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CIZ a Zinc Finger Protein That Interacts with p130cas and Activates the Expression of Matrix Metalloproteinases

机译:CIZ锌指蛋白与p130cas相互作用并激活基质金属蛋白酶的表达

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摘要

p130cas (Cas) is a docking protein that contains an SH3 domain and multiple tyrosine residues. p130cas is located at focal adhesions, is tyrosine phosphorylated in response to integrin stimulation, and is thought to transmit signals, via c-Crk and other proteins, for the remodeling of actin stress fibers and cell movement. In a search for the ligands of the SH3 domain of p130cas by far-Western screening, we cloned a novel protein named CIZ (for Cas-interacting zinc finger protein). CIZ consists of the following: a putative leucine zipper; a serine/threonine-rich region; a proline-rich sequence; five, six, or eight Krüppel-type C2H2 zinc fingers; and the glutamine-alanine repeat. CIZ binds Cas in cells and is located in the nucleus and at focal adhesions. We showed that CIZ is a nucleocytoplasmic shuttling protein, by using the transient interspecies heterokaryon formation assay. In order to search for the targets of CIZ in nucleus, we determined the DNA binding consensus of CIZ as (G/C)AAAAA(A) by cyclic amplification and selection of targets analysis. The consensus-like sequences are found in several promoters of matrix metalloproteinases (MMPs), which are the enzymes used to degrade the extracellular matrix proteins. CIZ binds to a consensus-like sequence in the MMP-1 (collagenase) promoter. Overexpression of CIZ upregulates the transcriptions from MMP-1, MMP-3 (stromelysin), and MMP-7 (matrilysin) promoters, and this transactivation was enhanced in the presence of Cas. Furthermore, the stable overexpression of CIZ promoted the production of MMP-7 in culture medium. In summary, CIZ, a novel zinc finger protein, binds Cas, is a nucleocytoplasmic shuttling protein, and regulates the expression of MMPs.
机译:p130 cas (Cas)是一个对接蛋白,其中包含一个SH3域和多个酪氨酸残基。 p130 cas 位于粘着斑处,在整合素刺激下酪氨酸被磷酸化,并被认为通过c-Crk和其他蛋白质传递信号,用于肌动蛋白应激纤维的重塑和细胞运动。为了通过远西筛选法搜索p130 cas 的SH3结构域的配体,我们克隆了一种新型蛋白CIZ(用于与Cas相互作用的锌指蛋白)。 CIZ由以下部分组成:假定的亮氨酸拉链;富含丝氨酸/苏氨酸的区域;富含脯氨酸的序列;五个,六个或八个Krüppel型C2H2锌指;和谷氨酰胺-丙氨酸重复。 CIZ结合细胞中的Cas,位于细胞核和粘着斑处。通过使用瞬时种间异核体形成分析,我们显示CIZ是一种核质穿梭蛋白。为了在细胞核中寻找CIZ的靶标,我们通过循环扩增和靶标选择的选择确定CIZ的DNA结合共识为(G / C)AAAAA(A)。在基质金属蛋白酶(MMP)的几种启动子中发现了共有样序列,这是用于降解细胞外基质蛋白的酶。 CIZ与MMP-1(胶原酶)启动子中的共有序列相似。 CIZ的过表达上调了MMP-1,MMP-3(基质溶素)和MMP-7(基质溶素)启动子的转录,这种反式激活在Cas存在下得以增强。此外,CIZ的稳定过表达促进了培养基中MMP-7的产生。总之,CIZ是一种新型锌指蛋白,与Cas结合,是一种核质穿梭蛋白,并调节MMP的表达。

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