Saviana B, Pons L, Namour F, Quilliot D, Ziegler O, Guéant J L
Laboratoire de Pathologie Cellulaire et Moléculaire en Nutrition, Equipe Mixte INSERM 00-14, Faculté de Médecome de Nancy, Vandoeuvre lès-Nancy, France.
J Chromatogr B Biomed Sci Appl. 2000 Jun 9;742(2):421-6. doi: 10.1016/s0378-4347(00)00155-9.
Quantitation of plasma apo B-48 is currently performed by densitometric analysis of SDS-PAGE zones stained with Coomassie Brilliant Blue, using standard solutions of purified apo B-48. Here, preparative gel electrophoresis with a continuous elution system was used for purifying apo B-48. A chylomicron fraction was isolated by 107,000 g ultracentrifugation of a chylous ascite. The proteins were delipidated and precipitated in ethanol-diethyl ether (3:1, v/v), subjected to preparative electrophoresis in a 5% polyacrylamide gel and eluted in 0.1% SDS. The peak containing apo B-48 was eluted at a retention time of 445-480 min. The purity of apo B-48 in this fraction was assessed by the detection of a single band (M(r) 260,000) after silver staining and Coomassie staining of 4-15% gradient SDS-PAGE. It was confirmed by the absence of apo B-100 contaminant in Western blot of the purified protein preparation. A linear relationship was observed between the densitometric analysis of SDS-PAGE bands and the apo B-48 in a protein range of 0-3 microg. In conclusion, preparative gel electrophoresis was used in a single step purification of apo B-48 that was adapted to the preparation of a standard solution.
目前,血浆载脂蛋白B-48的定量分析是通过用考马斯亮蓝染色的SDS-PAGE区域的光密度分析来进行的,使用纯化的载脂蛋白B-48标准溶液。在此,采用连续洗脱系统的制备性凝胶电泳来纯化载脂蛋白B-48。通过对乳糜腹水进行107,000g超速离心分离出乳糜微粒部分。蛋白质经脱脂后在乙醇-乙醚(3:1,v/v)中沉淀,在5%聚丙烯酰胺凝胶中进行制备性电泳,然后在0.1% SDS中洗脱。含有载脂蛋白B-48的峰在保留时间445 - 480分钟时洗脱。通过对4 - 15%梯度SDS-PAGE进行银染和考马斯染色后检测到单一条带(M(r) 260,000)来评估该部分中载脂蛋白B-48的纯度。通过对纯化蛋白质制剂进行Western印迹未检测到载脂蛋白B-100污染物来证实。在0 - 3μg蛋白质范围内,观察到SDS-PAGE条带的光密度分析与载脂蛋白B-48之间存在线性关系。总之,制备性凝胶电泳用于载脂蛋白B-48的单步纯化,该方法适用于标准溶液的制备。
