Arellano M, Coll P M, Yang W, Duran A, Tamanoi F, Perez P
Instituto de Microbiologia Bioquimica, CSIC/Universidad de Salamanca, Edificio Departamental, Spain.
Mol Microbiol. 1998 Sep;29(6):1357-67. doi: 10.1046/j.1365-2958.1998.01009.x.
The Schizosaccharomyces pombe cwg2+ gene encodes the beta-subunit of geranylgeranyl transferase I (GGTase I), which participates in the post-translational C-terminal modification of several small GTPases, allowing their targeting to the membrane. Using the two-hybrid system, we have identified the cwp1+ gene that encodes the alpha-subunit of the GGTase I. cwp1p interaction with cwg2p was mapped to amino acids 1-244 or 137-294 but was not restricted to amino acids 137-244. The genomic cwp1+ was isolated and sequenced. It has two putative open reading frames of 677 and 218 bp, separated by a 51 bp intron. The predicted amino acid sequence shows significant similarity to GGTase I alpha-subunits from different species. However, complementation of Saccharomyces cerevisiae ram2-1 mutant by overexpressing the cwp1+ gene was not possible. Expression of both cwg2+ and cwp1+ in Escherichia coli allowed 'in vitro' reconstitution of the GGTase I activity. S. pombe cells expressing the mutant enzyme containing the cwg2-1 mutation do not grow at 37 degrees C, but the growth defect can be suppressed by the addition of sorbitol. Actin immunostaining of the cwg2-1 mutant strain grown at 37 degrees C showed an abnormal distribution of actin patches. The cwg2-1 mutation was identified as a guanine to adenine substitution at nucleotide 604 of the coding region, originating the change A202T in the cwg2p. Deletion of the cwg2 gene is lethal; delta cwg2 spores can divide two or three times before losing viability. Most cells have aberrant morphology and septation defects. Overexpression of the rho1G15VC199R double-mutant allele in S. pombe caused loss of polarity but was not lethal and did not render the (1-3)beta-D-glucan synthase activity independent of GTP. Therefore, geranylgeranylation of rho1p is required for the appropriate function of this GTPase.
粟酒裂殖酵母cwg2⁺基因编码香叶基香叶基转移酶I(GGTase I)的β亚基,该酶参与几种小GTP酶的翻译后C末端修饰,使其能够靶向细胞膜。利用双杂交系统,我们鉴定出了编码GGTase Iα亚基的cwp1⁺基因。cwp1p与cwg2p的相互作用定位于氨基酸1 - 244或137 - 294,但不限于氨基酸137 - 244。分离并测序了基因组cwp1⁺。它有两个推定的开放阅读框,分别为677和218 bp,由一个51 bp的内含子隔开。预测的氨基酸序列与来自不同物种的GGTase Iα亚基具有显著相似性。然而,通过过表达cwp1⁺基因来互补酿酒酵母ram2 - 1突变体是不可能的。在大肠杆菌中同时表达cwg2⁺和cwp1⁺能够在“体外”重建GGTase I活性。表达含有cwg2 - 1突变的突变酶的粟酒裂殖酵母细胞在37℃下不能生长,但添加山梨醇可以抑制生长缺陷。对在37℃下生长的cwg2 - 1突变菌株进行肌动蛋白免疫染色,结果显示肌动蛋白斑分布异常。cwg2 - 1突变被鉴定为编码区核苷酸604处的鸟嘌呤到腺嘌呤的替换,导致cwg2p中发生A202T变化。缺失cwg2基因是致死的;δcwg2孢子在失去活力之前可以分裂两到三次。大多数细胞具有异常形态和隔膜缺陷。在粟酒裂殖酵母中过表达rho1G15VC199R双突变等位基因会导致极性丧失,但不具有致死性,也不会使(1 - 3)β - D - 葡聚糖合酶活性独立于GTP。因此,rho1p的香叶基香叶基化对于该GTP酶的正常功能是必需的。
