Micropreparative separation, fractionation, and peptide mapping of beta-lactoglobulin A and B variants by capillary electrophoresis.

Hector Armando Olguin-Arredondo, Belinda Vallejo-Cordoba, Aarón Fernando González-Córdova
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Abstract

The methodological aspects for the separation, fractionation, and peptide mapping by free zone capillary electrophoresis (CZE) of beta-lactoglobulin (beta-Lg) variants A and B were established. First, beta-Lg variants A or B were separated and fractionated by CZE. Then, the collected protein fraction was subjected to off-line tryptic digestion. Second, peptide mapping of the tryptic hydrolysates and peptide fraction collection were carried out by CZE. beta-Lg variants were separated and collected using an uncoated capillary (72 cm x 75 microm i.d.) in 0.05 M borate buffer containing 0.1% Tween 20 at pH 8.0 by applying 20 kV. By subjecting the capillary under pressure after a delay time of 15%, the protein was collected in a microvial containing digestion buffer. The most suitable conditions for the tryptic digestion of beta-Lg were established by monitoring the reaction products with CZE. A tryptic hydrolysis with an enzyme-to-substrate ratio (E/S) of 1/20 and incubation for 20 hr at 37 degrees C was found to result in the most suitable conditions. Peptides were separated and collected using an uncoated capillary (120 cm x 75 microm i.d.) in 0.15 M formic acid at pH 2.3 by applying 28 kV. Peptide maps were highly reproducible as shown by coefficients of variation of less than 0.89 and 5.42% for migration times and peak areas, respectively. Moreover, very good resolution of the peptide maps revealed the region in which the aberrant peptides of the beta-Lg variants may be located.

毛细管电泳对β -乳球蛋白A和B变异体的微制备分离、分离和多肽定位。
建立了β -乳球蛋白(β - lg)变体A和B的自由区毛细管电泳(CZE)分离、分离和肽定位的方法学方面。首先,用CZE分离和分馏β - lg变体A或B。然后,收集的蛋白质部分进行离线胰蛋白酶消化。其次,通过CZE对胰蛋白酶水解物进行肽图谱绘制和肽段收集。在含0.1% Tween 20的0.05 M硼酸盐缓冲液中,在pH 8.0下,施加20 kV,使用未涂膜毛细管(72 cm x 75 μ M id)分离和收集β - lg变体。延迟15%的时间后,毛细管受压,将蛋白质收集在含有消化缓冲液的微瓶中。通过CZE对反应产物的监测,确定了胰蛋白酶消化β - lg的最适宜条件。酶与底物比(E/S)为1/20,在37℃下孵育20小时的胰蛋白酶水解被发现是最合适的条件。肽分离和收集使用无包被毛细管(120 cm × 75 μ M id),在0.15 M甲酸中,pH为2.3,施加28 kV。迁移次数和峰面积的变异系数分别小于0.89和5.42%,表明肽图具有较高的重复性。此外,非常好的肽图分辨率揭示了β - lg变体的异常肽可能位于的区域。
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