Baboshina O V, Haas A L
Department of Biochemistry, Medical College of Wisconsin, Milwaukee 53226, USA.
J Biol Chem. 1996 Feb 2;271(5):2823-31. doi: 10.1074/jbc.271.5.2823.
Targeting of substrates for degradation by the ATP, ubiquitin-dependent pathway requires formation of multiubiquitin chains in which the 8.6-kDa polypeptide is linked by isopeptide bonds between carboxyl termini and Lys-48 residues of successive monomers. Binding of Lys-48-linked chains by subunit 5 of the 26 S proteasome regulatory complex commits the attached target protein to degradation with concomitant release of free ubiquitin monomers following disassembly of the chains. Point mutants of ubiquitin (Lys-->Arg) were used to map the linkage specificity for ubiquitin-conjugating enzymes previously demonstrated to form novel multiubiquitin chains not attached through Lys-48. Recombinant human E2EPF catalyzed multiubiquitin chain formation exclusively through Lys-11 of ubiquitin while recombinant yeast RAD6 formed chains linked only through Lys-6. Multiubiquitin chains linked through Lys-6, Lys-11, or Lys-48 each bound to subunit 5 of partially purified human 26 S proteasome with comparable affinities. Since chains bearing different linkages are expected to pack into distinct structures, competition between Lys-11 and Lys-48 chains for binding to subunit 5 demonstrates that the latter possesses determinants for recognizing alternatively linked chains and precludes the existence of subunit 5 isoforms recognizing distinct structures. In addition, competition studies provided an estimate of Kd < or = 18 nM for the intrinsic binding of Lys-48-linked chains of linkage number n > 4. This result suggests that the principal mechanistic advantage of multiubiquitin chain formation is to enhance the affinity of the associated substrate for the 26 S complex relative to that of unconjugated target protein. Complementation studies with E1/E2-depleted rabbit reticulocyte extract demonstrated RAD6 supported isopeptide ligase-dependent degradation only through Lys-48-linked chains, while E2EPF retained the ability to target a model radiolabeled substrate through Lys-11-linked chains. Therefore, the linkage specificity exhibited by these E2 isozymes depends on their catalytic context with respect to isopeptide ligase.
通过ATP依赖的泛素途径将底物靶向降解需要形成多聚泛素链,其中8.6 kDa的多肽通过连续单体的羧基末端与Lys-48残基之间的异肽键相连。26S蛋白酶体调节复合物的亚基5与Lys-48连接的链结合,使附着的靶蛋白降解,同时在链解离后释放游离的泛素单体。泛素的点突变体(Lys→Arg)用于绘制泛素结合酶的连接特异性图谱,该酶先前已被证明可形成不通过Lys-48连接的新型多聚泛素链。重组人E2EPF仅通过泛素的Lys-11催化多聚泛素链的形成,而重组酵母RAD6形成仅通过Lys-6连接的链。通过Lys-6、Lys-11或Lys-48连接的多聚泛素链各自以相当的亲和力与部分纯化的人26S蛋白酶体的亚基5结合。由于带有不同连接的链预计会堆积成不同的结构,Lys-11和Lys-48链之间与亚基5结合的竞争表明,后者具有识别交替连接链的决定因素,并排除了识别不同结构的亚基5同工型的存在。此外,竞争研究提供了对于连接数n>4的Lys-48连接链的内在结合的Kd≤18 nM的估计值。该结果表明,多聚泛素链形成的主要机制优势是相对于未缀合的靶蛋白增强相关底物对26S复合物的亲和力。用E1/E2耗尽的兔网织红细胞提取物进行的互补研究表明,RAD6仅通过Lys-48连接的链支持异肽连接酶依赖性降解,而E2EPF保留了通过Lys-11连接的链靶向模型放射性标记底物的能力。因此,这些E2同工酶表现出的连接特异性取决于它们相对于异肽连接酶的催化环境。
