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体内180-kD核糖体受体的功能特性

Functional characterization of the 180-kD ribosome receptor in vivo.

作者信息

Wanker E E, Sun Y, Savitz A J, Meyer D I

机构信息

Department of Biological Chemistry, UCLA School of Medicine 90024, USA.

出版信息

J Cell Biol. 1995 Jul;130(1):29-39. doi: 10.1083/jcb.130.1.29.

Abstract

A cDNA encoding the 180-kD canine ribosome receptor (RRp) was cloned and sequenced. The deduced primary structure indicates three distinct domains: an NH2-terminal stretch of 28 uncharged amino acids representing the membrane anchor, a basic region (pI = 10.74) comprising the remainder of the NH2-terminal half and an acidic COOH-terminal half (pI = 4.99). The most striking feature of the amino acid sequence is a 10-amino acid consensus motif, NQGKKAEGAP, repeated 54 times in tandem without interruption in the NH2-terminal positively charged region. We postulate that this repeated sequence represents a ribosome binding domain which mediates the interaction between the ribosome and the ER membrane. To substantiate this hypothesis, recombinant full-length ribosome receptor and two truncated versions of this protein, one lacking the potential ribosome binding domain, and one lacking the COOH terminus, were expressed in Saccharomyces cerevisiae. Morphological and biochemical analyses showed all proteins were targeted to, and oriented correctly in the ER membrane. In vitro ribosome binding assays demonstrated that yeast microsomes containing the full-length canine receptor or one lacking the COOH-terminal domain were able to bind two to four times as many human ribosomes as control membranes lacking a recombinant protein or microsomes containing a receptor lacking the NH2-terminal basic domain. Electron micrographs of these cells revealed that the expression of all receptor constructs led to a proliferation of perinuclear ER membranes known as "karmellae." Strikingly, in those strains which expressed cDNAs encoding a receptor containing the putative ribosome binding domain, the induced ER membranes (examined in situ) were richly studded with ribosomes. In contrast, karmellae resulting from the expression of receptor cDNA lacking the putative ribosome binding domain were uniformly smooth and free of ribosomes. Cell fractionation and biochemical analyses corroborated the morphological characterization. Taken together these data provide further evidence that RRp functions as a ribosome receptor in vitro, provide new evidence indicating its functionality in vivo, and in both cases indicate that the NH2-terminal basic domain is essential for ribosome binding.

摘要

克隆并测序了编码180-kD犬核糖体受体(RRp)的cDNA。推导的一级结构显示出三个不同的结构域:代表膜锚定的28个不带电荷的氨基酸的NH2末端延伸段、包含NH2末端后半部分的碱性区域(pI = 10.74)和酸性的COOH末端半段(pI = 4.99)。氨基酸序列最显著的特征是一个10个氨基酸的共有基序NQGKKAEGAP,在NH2末端带正电荷区域连续重复54次且无中断。我们推测这个重复序列代表一个核糖体结合结构域,介导核糖体与内质网(ER)膜之间的相互作用。为了证实这一假设,在酿酒酵母中表达了重组全长核糖体受体以及该蛋白的两个截短版本,一个缺少潜在的核糖体结合结构域,另一个缺少COOH末端。形态学和生化分析表明,所有蛋白质都靶向内质网膜并正确定向。体外核糖体结合试验表明,含有全长犬受体或缺少COOH末端结构域的酵母微粒体能够结合的人核糖体数量是缺少重组蛋白的对照膜或含有缺少NH2末端碱性结构域受体的微粒体的两到四倍。这些细胞的电子显微镜照片显示,所有受体构建体的表达都导致了称为“卡氏小体”的核周内质网膜的增殖。令人惊讶的是,在那些表达编码含有假定核糖体结合结构域受体的cDNA的菌株中,诱导的内质网膜(原位检查)上密集地布满了核糖体。相比之下,由于表达缺少假定核糖体结合结构域的受体cDNA而产生的卡氏小体表面均匀光滑且无核糖体。细胞分级分离和生化分析证实了形态学特征。这些数据综合起来进一步证明RRp在体外作为核糖体受体发挥作用,提供了其在体内功能的新证据,并且在这两种情况下都表明NH2末端碱性结构域对于核糖体结合至关重要。

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