Department of Cellular Biochemistry, Max-Planck-Institute for Biophysical Chemistry, Göttingen, Germany.
EMBO J. 2010 Dec 15;29(24):4172-84. doi: 10.1038/emboj.2010.295. Epub 2010 Nov 26.
U1 small nuclear ribonucleoprotein (snRNP) recognizes the 5'-splice site early during spliceosome assembly. It represents a prototype spliceosomal subunit containing a paradigmatic Sm core RNP. The crystal structure of human U1 snRNP obtained from natively purified material by in situ limited proteolysis at 4.4 Å resolution reveals how the seven Sm proteins, each recognize one nucleotide of the Sm site RNA using their Sm1 and Sm2 motifs. Proteins D1 and D2 guide the snRNA into and out of the Sm ring, and proteins F and E mediate a direct interaction between the Sm site termini. Terminal extensions of proteins D1, D2 and B/B', and extended internal loops in D2 and B/B' support a four-way RNA junction and a 3'-terminal stem-loop on opposite sides of the Sm core RNP, respectively. On a higher organizational level, the core RNP presents multiple attachment sites for the U1-specific 70K protein. The intricate, multi-layered interplay of proteins and RNA rationalizes the hierarchical assembly of U snRNPs in vitro and in vivo.
U1 小核核糖核蛋白 (snRNP) 在剪接体组装过程中早期识别 5'剪接位点。它代表了一种原型剪接体亚基,包含一个典范的 Sm 核心 RNP。通过在 4.4Å 分辨率下原位有限蛋白酶解从天然纯化的物质中获得的人 U1 snRNP 的晶体结构揭示了七个 Sm 蛋白如何使用它们的 Sm1 和 Sm2 基序识别 Sm 位点 RNA 的一个核苷酸。蛋白 D1 和 D2 引导 snRNA 进出 Sm 环,蛋白 F 和 E 介导 Sm 位点末端之间的直接相互作用。蛋白 D1、D2 和 B/B'的末端延伸以及 D2 和 B/B'中的扩展内部环分别支持四向 RNA 连接和 Sm 核心 RNP 两侧的 3'末端茎环。在更高的组织水平上,核心 RNP 呈现多个用于 U1 特异性 70K 蛋白的附着位点。蛋白质和 RNA 的复杂、多层次相互作用合理化了 U snRNP 在体外和体内的分层组装。
