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用焦谷氨酸氨肽酶高效去除重组免疫球蛋白氨基末端的封闭基团。

High-yield deblocking of amino termini of recombinant immunoglobulins with pyroglutamate aminopeptidase.

作者信息

Mozdzanowski J, Bongers J, Anumula K

机构信息

Bioanalytical Sciences, SmithKline Beecham Pharmaceuticals, King of Prussia, Pennsylvania 19406, USA.

出版信息

Anal Biochem. 1998 Jul 1;260(2):183-7. doi: 10.1006/abio.1998.2690.

Abstract

For larger proteins, efficient deblocking prior to Edman sequencing is especially important to obtain quality, extended sequencing data which is limited by the stepwise accumulation of background from the random acid hydrolysis of the protein. Therefore, any portion that remains blocked contributes to the undesirable background. We report an optimized procedure for the removal of pyroglutamate (pGlu) by pyroglutamate aminopeptidase (PGAP) and demonstrate its use for the quantitative deblocking of several humanized recombinant antibodies (rIgGs). The rIgGs with blocked heavy chain provided an advantageous system in which removal of pGlu from the heavy chain was determined as a ratio of the deblocked heavy chain to the light chain in the first cycle of sequencing; i.e., the light chain was used as an internal standard. The reaction temperature, reaction time, enzyme-to-substrate ratio, denaturation, and reduction/carboxymethylation prior to digestion, and different commercial enzymes were evaluated. The optimized procedure involves reduction/carboxymethylation in guanidine buffer, buffer exchange by gel-permeation chromatography, and overnight PGAP digestion at 37 degrees C. Five different rIgGs, including one with blocked heavy and light chains, were deblocked in nearly quantitative yields using this procedure.

摘要

对于较大的蛋白质,在进行埃德曼测序之前进行有效的去封闭尤为重要,以便获得高质量的、延伸的测序数据,因为蛋白质随机酸水解产生的背景会逐步累积,从而限制测序数据。因此,任何残留的封闭部分都会导致不理想的背景。我们报告了一种通过焦谷氨酸氨肽酶(PGAP)去除焦谷氨酸(pGlu)的优化方法,并展示了其用于几种人源化重组抗体(rIgG)定量去封闭的应用。带有封闭重链的rIgG提供了一个有利的系统,其中在测序的第一个循环中,从重链上去除pGlu的量以去封闭重链与轻链的比例来确定;即,轻链用作内标。对反应温度、反应时间、酶与底物的比例、消化前的变性以及还原/羧甲基化,以及不同的商业酶进行了评估。优化后的方法包括在胍缓冲液中进行还原/羧甲基化、通过凝胶渗透色谱进行缓冲液交换,以及在37℃下用PGAP消化过夜。使用该方法对五种不同的rIgG进行去封闭,包括一种重链和轻链均被封闭的rIgG,产率几乎达到定量。

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