Huang C F, Chuang N N
Department of Zoology, National Taiwan University and Institute of Zoology, Academia Sinica, Nankang, Taipei, Taiwan.
J Exp Zool. 2000 Apr 1;286(5):441-9. doi: 10.1002/(sici)1097-010x(20000401)286:5<441::aid-jez1>3.0.co;2-z.
In order to assess the effects of guanine nucleotide binding on the geranylgeranylation at the CAAX box of the shrimp Ras, we experimented with the shrimp Penaeus japonicus Ras (S-Ras) which is geranylgeranylated at the C-termini, shares 85% homology with mammalian K(B)-Ras protein and demonstrates identity in the guanine nucleotide binding domains (Huang C-F, Chuang N-N. 1999. J Exp Zool 283:510-521). Several point mutations in the S-ras gene were generated at codons 12 (G12V), 61 (Q61K), and 116 (N116I). The bacterially expressed mutant S-Ras proteins, G12V and Q61K, were bound with GTP without hydrolysis. In contrast, the mutant S-Ras N116I was defective in its ability to bind any guanine nucleotides. Autoradiography studies showed that the purified shrimp protein geranylgeranyltransferase I (Lin R-S, Chuang N-N. 1998. J Exp Zool 281:565-573) was unable to catalyze the transfer of [(3)H]-geranylgeranylpyrophosphate to this mutant N116I but very competently caused the geranylgeranylation of GTP-locked mutants, G12V and Q61K. These results demonstrate that the geranylgeranylation at the CAAX box of the shrimp Ras protein requires the proper binding of guanine nucleotide at its N-terminal region. J. Exp. Zool. 286:441-449, 2000.
为了评估鸟嘌呤核苷酸结合对虾Ras蛋白CAAX盒处香叶基香叶基化的影响,我们以日本对虾Ras(S-Ras)进行了实验,该蛋白在C末端进行香叶基香叶基化,与哺乳动物K(B)-Ras蛋白具有85%的同源性,并且在鸟嘌呤核苷酸结合结构域具有一致性(Huang C-F, Chuang N-N. 1999. J Exp Zool 283:510-521)。在S-ras基因的密码子12(G12V)、61(Q61K)和116(N116I)处产生了几个点突变。细菌表达的突变体S-Ras蛋白G12V和Q61K与GTP结合且不水解。相反,突变体S-Ras N116I结合任何鸟嘌呤核苷酸的能力存在缺陷。放射自显影研究表明,纯化的虾蛋白香叶基香叶基转移酶I(Lin R-S, Chuang N-N. 1998. J Exp Zool 281:565-573)无法催化将[(3)H]-香叶基香叶基焦磷酸转移到该突变体N116I上,但能非常有效地使GTP锁定的突变体G12V和Q61K发生香叶基香叶基化。这些结果表明,虾Ras蛋白CAAX盒处的香叶基香叶基化需要鸟嘌呤核苷酸在其N端区域的正确结合。《实验动物学杂志》286:441-449, 2000。
