Infante A A, Firshein W, Hobart P, Murray L
Biochemistry. 1976 Nov 2;15(22):4810-7. doi: 10.1021/bi00667a010.
A DNA-nuclear membrane complex has been isolated by two different methods from the nuclei of cultured mouse fibroblast (3T3) cells. One method, utilizing the detergent sarkosyl (sodium lauroyl sarkosinate), yields a DNA-nuclear membrane complex (the M band), which contains virtually all of the DNA in the nuclei. However, treatment of the M band by sonication, vortexing, or freeze-thaw reduces the amount of DNA in the complex by approximately 50-80%, depending upon the phase of the cell cycle from which the complex was extracted. The remaining DNA is tightly bound to the nuclear membrane and resists further shearing procedures. Over 90% of the choline-labeled phospholipid present in nuclei is also found in these sheared M bands. The percentage of DNA associated with the nuclear membrane varies during the cell cycle and correlates well with the onset, continuation, and cessation of DNA synthesis. Thus, although DNA-membrane complexes can be detected throughout the cell cycle, the percentage of DNA bound to membrane increases during late G1 and S and decreases during G2. In addition, there are distinct qualitative differences in the type of DNA present in the membrane fraction, with a more highly d(A-T) rich DNA being present in confluent (G0) cells than in cells during the S phase. This d(A-T) rich DNA may be related to the mouse satellite DNA identified by others. The M band can be separated into two DNA-nuclear membrane subfractions by centrifugation through a continuous sucrose gradient. The relative proportions of these two subfractions depend upon the percentage of sarkosyl present in the M band prior to centrifugation, with complete removal of sarkosyl resulting in a very large increase in the sedimentation velocity of the complex and in the formation of only one fraction. Evidence that this is a complex of DNA with membrane is given by the finding that DNA is dissociated from the complex with Pronase, deoxycholate, or high levels of sarkosyl. Removal of virtually all of the DNA with DNase from this rapidly sedimenting complex does not dissociate any of the phospholipid which still sediments rapidly as a single band. A second method, which yields a DNA-membrane fraction from nuclei, utilizes sedimentation of lysed nuclei to equilibrium in CsCl density gradients. This low-density CsCl fraction contains only 10-15% of the total DNA, but contains most of the nascent DNA, which may be chased into a membrane-free fraction. The DNA-membrane fraction from CsCl gradients possesses properties in common with the M-band fraction and can be converted into an M band. DNA membrane complexes from sucrose gradients, as well as the crude M-band preparation and a non-membrane-associated DNA fraction from nuclei can synthesize DNA in vitro without the addition of an external DNA template or DNA polymerase. In contrast to the activity in the non-membrane-associated DNA fraction, the membrane-associated polymerase activity is strongly stimulated by adenosine triphosphate and is unaffected by ethidium bromide...
已通过两种不同方法从培养的小鼠成纤维细胞(3T3)细胞核中分离出一种DNA-核膜复合物。一种方法是利用去污剂 Sarkosyl(月桂酰肌氨酸钠),得到一种DNA-核膜复合物(M带),它几乎包含了细胞核中的所有DNA。然而,通过超声处理、涡旋或冻融处理M带,复合物中的DNA量会减少约50%-80%,这取决于提取复合物时细胞周期的阶段。剩余的DNA与核膜紧密结合,抵抗进一步的剪切程序。细胞核中超过90%的胆碱标记磷脂也存在于这些剪切后的M带中。与核膜相关的DNA百分比在细胞周期中会发生变化,并且与DNA合成的开始、持续和停止密切相关。因此,尽管在整个细胞周期中都能检测到DNA-膜复合物,但与膜结合的DNA百分比在G1晚期和S期增加,在G2期减少。此外,膜部分中存在的DNA类型存在明显的定性差异,汇合(G0)细胞中富含d(A-T)的DNA比S期细胞中的更多。这种富含d(A-T)的DNA可能与其他人鉴定的小鼠卫星DNA有关。通过在连续蔗糖梯度中离心,M带可分为两个DNA-核膜亚组分。这两个亚组分的相对比例取决于离心前M带中Sarkosyl的百分比,完全去除Sarkosyl会导致复合物的沉降速度大幅增加,并仅形成一个组分。用链霉蛋白酶、脱氧胆酸盐或高浓度的Sarkosyl可使DNA从复合物中解离,这一发现证明这是一种DNA与膜的复合物。用DNase从这种快速沉降的复合物中去除几乎所有的DNA,不会使任何磷脂解离,这些磷脂仍作为一个单一的带快速沉降。从细胞核中获得DNA-膜部分的第二种方法是利用裂解细胞核在CsCl密度梯度中沉降至平衡。这个低密度的CsCl部分仅包含总DNA的10%-15%,但包含大部分新生DNA,这些新生DNA可被追踪到一个无膜部分。来自CsCl梯度的DNA-膜部分具有与M带部分共同的特性,并且可以转化为M带。来自蔗糖梯度的DNA膜复合物,以及粗制的M带制剂和细胞核中与膜无关的DNA部分,在不添加外部DNA模板或DNA聚合酶的情况下,可在体外合成DNA。与与膜无关的DNA部分的活性相反,与膜相关的聚合酶活性受到三磷酸腺苷的强烈刺激,并且不受溴化乙锭的影响……
