山西医科大学学报
山西醫科大學學報
산서의과대학학보
JOURNAL OF SHANXI MEDICAL UNIVERSITY
2005年
4期
395-398
,共4页
封启龙%范国权%赵嘉惠%赵画晨%吴博威
封啟龍%範國權%趙嘉惠%趙畫晨%吳博威
봉계룡%범국권%조가혜%조화신%오박위
钠-钙交换体%α-1重复序列%α-2重复序列
鈉-鈣交換體%α-1重複序列%α-2重複序列
납-개교환체%α-1중복서렬%α-2중복서렬
sodium-calcium exchanger%α-1 repeat%α-2 repeat
目的用人工合成的钠-钙交换体α-1和α-2重复序列作为抗原,制备并纯化抗α-1和α-2重复序列抗体.方法通过主动免疫大鼠,获得抗血清.采用酶联免疫吸附测定法(SA-ELISA) 测定抗体滴度,并将高滴度抗血清(≥1∶640)上样至HiTrap Protein G HP 进行亲和层析对抗体进行纯化.纯化效果用非变性聚丙烯酰胺凝胶电泳检测,并采用Bradford蛋白质定量法对纯化后抗体进行定量.结果大鼠经主动免疫后,抗α-1抗血清滴度从免疫前的1∶(25.5±1.5)升高到1∶(905.1±2.2)(P<0.01);抗α-2抗血清滴度从免疫前的1∶(26.4±1.5)升高到1∶(1 076.3±2.0)(P<0.01).纯化后的抗α-1和抗α-2重复序列抗体电泳时都仅有一条带出现,分子量160 kDa左右,与IgG标准品相一致.用Bradford蛋白质定量法测得抗α-1和α-2抗体浓度分别为1.0 mg/ml和1.2 mg/ml. 结论本研究获得了高纯度、高滴度的抗α-1抗体,为下一步对其进行功能研究奠定了基础.
目的用人工閤成的鈉-鈣交換體α-1和α-2重複序列作為抗原,製備併純化抗α-1和α-2重複序列抗體.方法通過主動免疫大鼠,穫得抗血清.採用酶聯免疫吸附測定法(SA-ELISA) 測定抗體滴度,併將高滴度抗血清(≥1∶640)上樣至HiTrap Protein G HP 進行親和層析對抗體進行純化.純化效果用非變性聚丙烯酰胺凝膠電泳檢測,併採用Bradford蛋白質定量法對純化後抗體進行定量.結果大鼠經主動免疫後,抗α-1抗血清滴度從免疫前的1∶(25.5±1.5)升高到1∶(905.1±2.2)(P<0.01);抗α-2抗血清滴度從免疫前的1∶(26.4±1.5)升高到1∶(1 076.3±2.0)(P<0.01).純化後的抗α-1和抗α-2重複序列抗體電泳時都僅有一條帶齣現,分子量160 kDa左右,與IgG標準品相一緻.用Bradford蛋白質定量法測得抗α-1和α-2抗體濃度分彆為1.0 mg/ml和1.2 mg/ml. 結論本研究穫得瞭高純度、高滴度的抗α-1抗體,為下一步對其進行功能研究奠定瞭基礎.
목적용인공합성적납-개교환체α-1화α-2중복서렬작위항원,제비병순화항α-1화α-2중복서렬항체.방법통과주동면역대서,획득항혈청.채용매련면역흡부측정법(SA-ELISA) 측정항체적도,병장고적도항혈청(≥1∶640)상양지HiTrap Protein G HP 진행친화층석대항체진행순화.순화효과용비변성취병희선알응효전영검측,병채용Bradford단백질정량법대순화후항체진행정량.결과대서경주동면역후,항α-1항혈청적도종면역전적1∶(25.5±1.5)승고도1∶(905.1±2.2)(P<0.01);항α-2항혈청적도종면역전적1∶(26.4±1.5)승고도1∶(1 076.3±2.0)(P<0.01).순화후적항α-1화항α-2중복서렬항체전영시도부유일조대출현,분자량160 kDa좌우,여IgG표준품상일치.용Bradford단백질정량법측득항α-1화α-2항체농도분별위1.0 mg/ml화1.2 mg/ml. 결론본연구획득료고순도、고적도적항α-1항체,위하일보대기진행공능연구전정료기출.
Objective To raise and purify antibodies against the synthesized α-1 repeat and α-2 repeat. Methods The rats were actively immunized with synthesized α-1 and α-2 repeats.Titer of the antibodies was determined by SA-ELISA.To diminish the undesired effects of other proteins than immunoglobulin,especially serum albumin,the positive antisera with high titer (≥1∶640) were applied on the HiTrap protein G HP column which was an affinity chromatography column for purification of IgG from serum.The purity of the antibodies was tested by PAGE in nonreducing condition and the concentrations of the antibodies were determined by the protein quantification method described by Bradford. Results ① Titers of antibodies against α-1 repeat and α-2 repeat in both immunized groups differed largely among different rats and increased from 1∶(25.5±1.5) and (26.4±1.5) before immunization to 1∶(905.1±2.2) and (1 076.3±2.0) (P<0.01) after the second booster immunization,respectively.②From the results of PAGE in nonreducing condition,only one band with the same molecular weight as standard IgG could be seen in the samples of the purified antibodies against α-1 repeat and α-2 repeat.③The concentrations of the antibodies against α-1 repeat and α-2 repeat were about 1.0 mg/ml and 1.2 mg/ml respectively by the Bradford assay. Conclusion Antibodies against the synthesized α-1 repeat and α-2 repeat are successfully raised and purified,providing a basis for further investigation on their function.