Division of Biological Sciences, Section of Cell and Developmental Biology, University of California, San Diego, La Jolla, California 92093-0347, USA.
J Biol Chem. 2009 Dec 18;284(51):35368-80. doi: 10.1074/jbc.M109.023994.
3-Hydroxy-3-methylglutaryl (HMG)-CoA reductase (HMGR), the rate-limiting enzymes of sterol synthesis, undergoes feedback-regulated endoplasmic reticulum degradation in both mammals and yeast. The yeast Hmg2p isozyme is subject to ubiquitin-mediated endoplasmic reticulum degradation by the HRD pathway. We had previously shown that alterations in cellular levels of the 15-carbon sterol pathway intermediate farnesyl pyrophosphate (FPP) cause increased Hmg2p ubiquitination and degradation. We now present evidence that the FPP-derived, 20-carbon molecule geranylgeranyl pyrophosphate (GGPP) is a potent endogenous regulator of Hmg2p degradation. This work was launched by the unexpected observation that GGPP addition directly to living yeast cultures caused high potency and specific stimulation of Hmg2p degradation. This effect of GGPP was not recapitulated by FPP, GGOH, or related isoprenoids. GGPP-caused Hmg2p degradation met all the criteria for the previously characterized endogenous signal. The action of added GGPP did not require production of endogenous sterol molecules, indicating that it did not act by causing the build-up of an endogenous pathway signal. Manipulation of endogenous GGPP by several means showed that naturally made GGPP controls Hmg2p stability. Analysis of the action of GGPP indicated that the molecule works upstream of retrotranslocation and can directly alter the structure of Hmg2p. We propose that GGPP is the FPP-derived regulator of Hmg2p ubiquitination. Intriguingly, the sterol-dependent degradation of mammalian HMGR is similarly stimulated by the addition of GGOH to intact cells, implying that a dependence on 20-carbon geranylgeranyl signals may be a common conserved feature of HMGR regulation that may lead to highly specific therapeutic approaches for modulation of HMGR.
3-羟-3-甲基戊二酰辅酶 A(HMG)-CoA 还原酶(HMGR)是固醇合成的限速酶,在哺乳动物和酵母中均经历受反馈调节的内质网降解。酵母 Hmg2p 同工酶通过 HRD 途径受到泛素介导的内质网降解。我们之前曾表明,细胞内 15-碳甾醇途径中间产物法呢基焦磷酸(FPP)水平的改变会导致 Hmg2p 泛素化和降解增加。我们现在提供的证据表明,FPP 衍生的 20-碳分子香叶基香叶基焦磷酸(GGPP)是 Hmg2p 降解的有效内源性调节剂。这项工作的启动是由于一个意外的观察结果,即 GGPP 直接添加到活酵母培养物中会导致 Hmg2p 降解的高效力和特异性刺激。这种 GGPP 的作用不能被 FPP、GGOH 或相关异戊二烯类物质再现。GGPP 引起的 Hmg2p 降解符合之前描述的内源性信号的所有标准。添加 GGPP 的作用不需要产生内源性固醇分子,这表明它不是通过引起内源性途径信号的积累而起作用的。通过几种方法对内源性 GGPP 的操作表明,天然产生的 GGPP 控制 Hmg2p 的稳定性。对 GGPP 作用的分析表明,该分子在上游逆转录后作用,并且可以直接改变 Hmg2p 的结构。我们提出 GGPP 是 Hmg2p 泛素化的 FPP 衍生调节剂。有趣的是,添加 GGOH 到完整细胞中同样会刺激哺乳动物 HMGR 的固醇依赖性降解,这意味着对 20-碳香叶基香叶基信号的依赖可能是 HMGR 调节的一个常见保守特征,这可能导致 HMGR 调节的高度特异性治疗方法。