Lin L N, Brandts J F
Biochemistry. 1984 Nov 20;23(24):5713-23. doi: 10.1021/bi00319a009.
Using the method of isomer-specific proteolysis (ISP), the cis-trans nature of the peptide bonds involving prolines-114 and -117 in ribonuclease (RNase) has been investigated. These studies involve the pretreatment of RNase first with either a short pepsin pulse or a short mercaptoethanol pulse to irreversibly unfold the protein and then with a short chymotrypsin pulse to quickly cleave the Tyr115-Val116 bond so that the chain is suitably trimmed for the subsequent stereospecific cleavage either by aminopeptidase P, to investigate proline-117, or by a proline-specific endopeptidase, to investigate proline-114. The most reasonable interpretation of our results suggests that proline-117 is essentially 100% trans in both the native and unfolded states, so it apparently makes no direct contribution to the slow refolding kinetics of RNase. It is also determined that proline-114 is 100% cis in native RNase and ca. 95% cis in reversibly unfolded RNase so only 5% of the unfolded RNase can be rate limited by trans to cis isomerization of proline-114 during refolding. Careful spectroscopic studies of refolding show that the smallest and slowest of the refolding phases, the ct phase, has the proper amplitude (5%), relaxation time (400 s at 10 degrees C), and activation energy (17 kcal) for a phase that is rate limited by the trans to cis isomerization of proline-114. Measurements of the kinetics of binding of cytidine 2'-monophosphate during refolding further show that RNase does not become active until proline-114 has isomerized to the native cis configuration. It is concluded that none of the three prolines thus far examined (i.e., prolines-93, -114, and -117) by the ISP method is involved in the formation of a fully active, nativelike intermediate which has "incorrect" proline isomers. The specific structural process which is responsible for the largest of the three slow refolding phases, the XY phase, is still undetermined. Although ISP results on proline-42 are not yet available, it seems possible that this slow phase may be rate limited by a process other than proline isomerization. In unrelated studies, results from chymotrypsin hydrolyses of several short peptides containing the sequence -X-Y-Pro- show that cleavage of an active X-Y bond is very slow when it is immediately adjacent on the amino side of a proline peptide bond. Thus, chymotrypsin cleavage may not be generally useful as the analytical step in isomer-specific proteolysis.
运用异构体特异性蛋白水解法(ISP),对核糖核酸酶(RNase)中涉及脯氨酸-114和-117的肽键的顺反性质进行了研究。这些研究包括先用短时间的胃蛋白酶脉冲或短时间的巯基乙醇脉冲对RNase进行预处理,以使蛋白质不可逆地展开,然后用短时间的胰凝乳蛋白酶脉冲快速切割Tyr115-Val116键,从而使链适当缩短,以便后续通过氨肽酶P进行立体特异性切割来研究脯氨酸-117,或通过脯氨酸特异性内肽酶来研究脯氨酸-114。对我们结果最合理的解释表明,脯氨酸-117在天然状态和未折叠状态下基本上都是100%反式,因此它显然对RNase缓慢的重折叠动力学没有直接贡献。还确定脯氨酸-114在天然RNase中是100%顺式,在可逆展开的RNase中约为95%顺式,所以在重折叠过程中,只有5%的未折叠RNase可能受脯氨酸-114从反式到顺式异构化的速率限制。对重折叠的仔细光谱研究表明,重折叠阶段中最小且最慢的ct阶段,其幅度(5%)、弛豫时间(10℃时为400秒)和活化能(17千卡)对于一个受脯氨酸-114从反式到顺式异构化速率限制的阶段来说是合适的。对重折叠过程中胞苷2'-单磷酸结合动力学的测量进一步表明,直到脯氨酸-114异构化为天然顺式构型,RNase才会变得有活性。得出的结论是,迄今为止通过ISP方法检测的三个脯氨酸(即脯氨酸-93、-114和-117)中,没有一个参与形成具有“错误”脯氨酸异构体的完全活性、类似天然状态的中间体。导致三个缓慢重折叠阶段中最大阶段XY的具体结构过程仍未确定。尽管关于脯氨酸-42的ISP结果尚未可得,但似乎这个缓慢阶段可能受脯氨酸异构化以外的过程的速率限制。在无关研究中,对几个含有序列-X-Y-Pro-的短肽进行胰凝乳蛋白酶水解的结果表明,当活性X-Y键紧邻脯氨酸肽键的氨基侧时,其切割非常缓慢。因此,胰凝乳蛋白酶切割作为异构体特异性蛋白水解中的分析步骤可能一般并不有用。
