Nguyen-Gia P, Bomsel M, Labrousse J P, Gallien C L, Weintraub H
Eur J Biochem. 1986 Dec 15;161(3):771-7. doi: 10.1111/j.1432-1033.1986.tb10506.x.
A 200-fold purification of the maturation-promoting factor or MPF from unfertilized eggs of Xenopus laevis is reported for the first time. Purification was achieved by three successive column chromatographies on hydroxyapatite, trisacryl blue and L-arginine-agarose. The presence of MPF was assessed by the usual maturation criteria after injections of test material into immature stage VI unstimulated X. laevis oocytes: the precocious appearance of the maturation spot (within 45-120 min), the germinal vesicle breakdown, the presence of the first polar body and the second metaphase spindle. Purification was monitored by the decrease of the minimal amount of protein injected in a constant volume (50 nl) required to induce 50% frequency of germinal vesicle breakdown. This amount decreased from 500 ng in the crude extract to 2.5 ng in the 200-fold purified material. Analysis by SDS-PAGE of the crude extract showed about 40 Coomassie-blue-stained polypeptides with molecular masses ranging from 300 kDa to 20 kDa, whereas in the 200-fold purified MPF only 5 stained polypeptides were revealed, with molecular masses of 62, 53, 49, 39 and 37 kDa. In vitro phosphorylations for the detection of kinase activities for endogenous and exogenous substrates were monitored by analysis of autoradiograms of SDS-PAGE, after treatment of fractions with [gamma-32P]ATP. Only inactive fractions eluted from columns ahead of MPF, and fractions containing MPF activity were tested. Phosphorylation of numerous stained polypeptides was demonstrated in the crude MPF extract and exogenous substrates such as phosvitin, casein and histone type II-AS were also strongly phosphorylated. In the MPF fraction, purified on hydroxyapatite, a polypeptide of 53 kDa was more highly and specifically phosphorylated and the presence of kinase activities was observed for the above three exogenous substrates. In the 100-fold and 200-fold purified MPF, phosphorylation of endogenous substrates could not be shown and kinase activities for the above three substrates were drastically decreased as compared with the crude and purified MPF obtained after hydroxyapatite column chromatography. However, neither endogenous phosphorylations nor kinase activities with the above exogenous substrates could be shown in inactive fractions eluted ahead of MPF at the different purification steps. Some characteristics of the purified material are also described in this paper.
首次报道了从非洲爪蟾未受精卵中对成熟促进因子(MPF)进行200倍的纯化。通过在羟基磷灰石、三丙烯酸蓝和L-精氨酸琼脂糖上进行三次连续柱层析实现了纯化。将测试材料注射到未受刺激的第VI期未成熟非洲爪蟾卵母细胞中后,通过常规的成熟标准评估MPF的存在:成熟斑早熟出现(45 - 120分钟内)、生发泡破裂、第一极体的存在以及第二中期纺锤体的存在。通过降低在恒定体积(50 nl)中诱导50%生发泡破裂频率所需注射的最小蛋白量来监测纯化过程。该量从粗提物中的500 ng降至200倍纯化材料中的2.5 ng。对粗提物进行SDS-PAGE分析显示约有40条考马斯亮蓝染色的多肽,分子量范围从300 kDa到20 kDa,而在200倍纯化的MPF中仅显示5条染色多肽,分子量分别为62、53、49、39和37 kDa。在用[γ-32P]ATP处理各组分后,通过分析SDS-PAGE的放射自显影片来监测用于检测内源性和外源性底物激酶活性的体外磷酸化。仅对从柱上在MPF之前洗脱的无活性组分以及含有MPF活性的组分进行了测试。在粗MPF提取物中证实了许多染色多肽的磷酸化,并且外源性底物如卵黄高磷蛋白、酪蛋白和II - AS型组蛋白也被强烈磷酸化。在经羟基磷灰石纯化的MPF组分中,一条53 kDa的多肽被更高度且特异性地磷酸化,并且观察到上述三种外源性底物存在激酶活性。在100倍和200倍纯化的MPF中,未显示内源性底物的磷酸化,并且与经羟基磷灰石柱层析获得的粗MPF和纯化MPF相比,上述三种底物的激酶活性急剧降低。然而,在不同纯化步骤中在MPF之前洗脱的无活性组分中,既未显示内源性磷酸化,也未显示与上述外源性底物的激酶活性。本文还描述了纯化材料的一些特性。
