Waheed A, Shadduck R K
J Lab Clin Med. 1979 Jul;94(1):180-93.
CSF was prepared by the growth of L cells in serum-free culture medium. This conditioned medium was subjected to a six-step purification schedule which included ultrafiltration, alcohol precipitation, and separation by DEAE-cellulose, Con A-Sepharose, Sephadex G-150, and sucrose density-gradient centrifugation. The resultant CSF was 1000-fold purified with 50% to 70% recovery of the starting activity. Granulocyte and macrophage colony formation was detected with 5 x 10(-12M CSF; maximum colonies were obtained with 3 ng per marrow culture. Two major peaks of activity were obtained; one was nonadherent to Con A, whereas the other was bound and specifically eluted with alpha-methylglucoside. Both fractions contained carbohydrate residues as they stained avidly with PAS, were inactivated by periodate, and showed altered electrophoretic mobility after treatment with neuraminidase. Following iodination, each purified fraction migrated in a single band in SDS-acrylamide gels. The molecular weight was estimated as 65,000 to 70,000 daltons. Following reduction with mercaptoethanol, the CSF fractions were reduced into subunits with molecular weights of approximately 35,000. These studies confirm the glycoprotein nature and subunit composition of L cell CSF. The methods described herein are useful for the purification of both the Con A-adherent and con A-nonadherent forms of CSF.
通过在无血清培养基中培养L细胞来制备集落刺激因子(CSF)。将这种条件培养基进行六步纯化程序,包括超滤、乙醇沉淀,以及通过DEAE-纤维素、伴刀豆球蛋白A-琼脂糖凝胶、葡聚糖凝胶G-150和蔗糖密度梯度离心进行分离。最终得到的CSF纯化了1000倍,起始活性回收率为50%至70%。用5×10⁻¹²M的CSF可检测到粒细胞和巨噬细胞集落形成;每骨髓培养物中加入3 ng可获得最大集落数。得到了两个主要的活性峰;一个不与伴刀豆球蛋白A结合,而另一个与之结合并能用α-甲基葡萄糖苷特异性洗脱。两个组分都含有碳水化合物残基,因为它们与过碘酸希夫(PAS)试剂强烈染色,被高碘酸盐灭活,并且在用神经氨酸酶处理后电泳迁移率发生改变。碘化后,每个纯化组分在SDS-丙烯酰胺凝胶中迁移为单一条带。估计分子量为65,000至70,000道尔顿。用巯基乙醇还原后,CSF组分被还原为分子量约为35,000的亚基。这些研究证实了L细胞CSF的糖蛋白性质和亚基组成。本文所述方法可用于纯化CSF的伴刀豆球蛋白A结合型和非结合型。
