Schnaar R I, Schaffner A E
J Neurosci. 1981 Feb;1(2):204-17. doi: 10.1523/JNEUROSCI.01-02-00204.1981.
Single cell suspensions prepared from embryonic chick or rat spinal cords were separated into morphologically and functionally distinct subpopulation based on their buoyant densities The lightest fraction (F-1) was highly enriched for cells containing the enzyme choline acetyltransferase (CAT), a marker for developing motoneurons. The morphology biochemistry, and in vitro development of this and other spinal cord cell fractions isolated by the outlined procedure were investigated. Spinal cords, dissected from 6-day chick or 12-day rat embryos, were dissociated with trypsin and applied to iso-osmotic metrizamide density gradients. After brief centrifugation, biochemical analysis revealed that cholinergic cells migrated to lower densities than other spinal cord cells. The use of discontinuous density gradients allowed rapid and simple isolation of three fractions of viable cells (designated F-1 to F-3, lowest to highest density). Characterization of chicken and rat embryo cell fractions gave similar results. The cells in Fraction 1 were large with prominent nuclei and nucleoli, while those in F-2 and F-3 were distinctly smaller. Fraction 1 was highly enriched for cholinergic cells. The CAT specific activity (CAT/cell) was increased 400% in Fraction 1 compared to unfractionated cells, while CAT specific activity in F-2 and F-3 was reduced to 25% and less than 4% that of unfractionated cells, respectively. The recovery of cholinergic cells using this procedure was much better than with other published procedures; greater than half the spinal cord CAT activity was routinely recovered in the enriched fraction. The cholinergic-enriched cells (F-1) were unique in their in vitro growth characteristics. All fractions had neuronal cells, while non-neuronal cells were distributed primarily in F-3, fewer in F-2, and were essentially absent from F-1. Neurons in F-2 and F-3 remained viable under a variety of conditions, most of which were not supportive of F-1 cell survival. The cholinergic-enriched F-1 cells survived and developed only in the presence of muscle cells or in muscle-conditioned medium on highly adhesive substrata. Large, multipolar neurons predominated under these conditions. The method described provides a means of characterizing the factors involved in the development of distinct populations of cells from the embryonic spinal cord.
从胚胎期鸡或大鼠脊髓制备的单细胞悬液,根据其浮力密度被分离成形态和功能上不同的亚群。最轻的部分(F-1)高度富集了含有胆碱乙酰转移酶(CAT)的细胞,CAT是发育中的运动神经元的标志物。对通过上述方法分离的该部分及其他脊髓细胞部分的形态、生物化学和体外发育进行了研究。从6日龄鸡或12日龄大鼠胚胎中取出的脊髓,用胰蛋白酶解离后应用于等渗的甲泛葡胺密度梯度。短暂离心后,生化分析表明胆碱能细胞迁移到比其他脊髓细胞更低的密度区域。使用不连续密度梯度可快速简单地分离出三部分活细胞(分别命名为F-1至F-3,密度从低到高)。对鸡和大鼠胚胎细胞部分的特征分析得到了相似的结果。F-1部分的细胞较大,细胞核和核仁突出,而F-2和F-3部分的细胞明显较小。F-1部分高度富集胆碱能细胞。与未分离的细胞相比,F-1部分的CAT比活性(CAT/细胞)增加了400%,而F-2和F-3部分的CAT比活性分别降至未分离细胞的25%和不到4%。使用该方法回收胆碱能细胞的效果比其他已发表的方法要好得多;在富集部分中,通常能回收超过一半的脊髓CAT活性。富含胆碱能的细胞(F-1)在体外生长特性方面具有独特性。所有部分都有神经元细胞,而非神经元细胞主要分布在F-3部分,F-2部分较少,F-1部分基本没有。F-2和F-3部分的神经元在各种条件下都能存活,其中大多数条件不支持F-1细胞存活。富含胆碱能的F-1细胞仅在肌肉细胞存在或在高黏附性基质上的肌肉条件培养基中存活并发育。在这些条件下,大型多极神经元占主导。所描述的方法提供了一种表征参与胚胎脊髓中不同细胞群体发育的因素的手段。