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用钴(Ⅲ)螯合物对肽和蛋白质的N端氨基酸进行定性测定。

Qualitative determination of N-terminal amino acids of peptides and proteins with cobalt(3) chelates.

作者信息

Bentley K W, Creaser E H

出版信息

Biochem J. 1973 Nov;135(3):507-11. doi: 10.1042/bj1350507.

Abstract
  1. A method of N-terminal peptide-bond hydrolysis with the cis-beta-hydroxyaquo(triethylenetetramine)cobalt(III) ion, i.e. beta-Co(trien)(OH)(OH(2)), is reported. The method has been demonstrated with 22 small peptides and ten proteins. 2. The procedure is rapid (an N-terminal amino acid determination can be made easily in one day), it involves no acid hydrolysis step and thus no destruction of labile amino acids, and it involves the use of easily prepared inexpensive reagents. 3. The released N-terminal amino acids can be identified as their cobalt(III) derivatives, or directly as the amino acid or as their dansylated derivatives. 4. The method is to treat 1 mumol of peptide or protein with beta-Co(trien)(OH)(OH(2)) reagent at pH8.0, 45 degrees C for 3h. Addition of 0.5m-phosphate buffer, pH10.5 at 45 degrees C for 10min cleaves the N-terminal bidentate amino acid-cobalt complex, which can be identified directly. For greater sensitivity with 10nmol of peptide) the free amino acid is prepared from the complex by treatment (with NaCN (0.1m, 40 degrees C, 30min), or H(2)S or NaBH(4) (25 degrees C, 5min), dried, dansylated and the dansyl-amino acid identified by high-voltage electrophoresis. The method is unaffected by the presence of 4-8m-urea, but will not cleave blocked N-terminal acids.
摘要
  1. 报道了一种用顺式-β-羟基水合(三亚乙基四胺)钴(III)离子,即β-[Co(trien)(OH)(OH₂)]²⁺进行N端肽键水解的方法。该方法已在22种小肽和10种蛋白质上得到验证。2. 该方法快速(一天内可轻松完成N端氨基酸测定),不涉及酸水解步骤,因此不会破坏不稳定氨基酸,且使用的试剂易于制备且价格低廉。3. 释放的N端氨基酸可鉴定为其钴(III)衍生物,或直接鉴定为氨基酸或其丹磺酰化衍生物。4. 该方法是将1 μmol肽或蛋白质与β-[Co(trien)(OH)(OH₂)]²⁺试剂在pH8.0、45℃下处理3小时。加入0.5m磷酸缓冲液,在45℃、pH10.5下处理10分钟可裂解N端双齿氨基酸-钴络合物,可直接鉴定。对于10 nmol肽,为提高灵敏度,可通过用NaCN(0.1m,40℃,30分钟)或H₂S或NaBH₄(25℃,5分钟)处理从络合物中制备游离氨基酸,干燥,丹磺酰化,然后通过高压电泳鉴定丹磺酰氨基酸。该方法不受4-8m尿素存在的影响,但不能裂解封闭的N端酸。

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