Barald K F
Department of Anatomy, University of Michigan Medical School, Ann Arbor 48109.
Dev Biol. 1989 Oct;135(2):349-66. doi: 10.1016/0012-1606(89)90185-1.
Although neural crest cells are known to be very responsive to environmental cues during their development, recent evidence indicates that at least some subpopulations may be committed to a specific differentiation program prior to migration. Because the neural crest is composed of a heterogeneous mixture of cells that contributes to many vertebrate cell lineages, assessing the properties of specific subpopulations and the effect of the environment on their development has been difficult. To address this problem, we have isolated a pure subpopulation of chick mesencephalic neural crest cells by fluorescence no-flow cytometry after labeling them with monoclonal antibodies (Mabs) to a 75-kDa cell surface antigen that is associated with high affinity choline uptake. When cultures of chick mesencephalic neural crest cells are labeled with these Mabs and a fluorescent second step antibody, approximately 5% of the cells are antigen-positive (A+). After sorting, 100% of the resulting cultured mesencephalic neural crest cells are A+. The Mabs we used also label all of the neurons of the embryonic chick and quail ciliary ganglion in vivo and in vitro. We have compared the effect of various cell culture media on the isolated neural crest subpopulation and the heterogeneous chick mesencephalic neural crest from which it was derived. A+ cells were passaged and grown in a variety of media, each of which differently affected its characteristics and development. A+ cells proliferated in the presence of 15% fetal bovine serum (FBS) and high concentrations (10-15%) of chick embryo extract, but did not differentiate, although they retained basal levels of choline acetyltransferase (ChAT) activity. However, in chick serum and high (25 mM as opposed to 7 mM) K+, and heart-, iris-, or lung-conditioned medium, all of which are known to promote survival and/or cholinergic development of ciliary ganglion neurons, the cells ceased to proliferate and all of the cells in the culture became "neuron-like" within 10 days. No neuron-like cells were found in liver-, notocord-, or neural tube-conditioned media if FBS was used. When A+ cells were eliminated either by complement-mediated cytotoxicity or by laser-ablating A+ cells during no-flow cytometry, all ChAT activity was also eliminated, and no neuron-like cells or ChAT activity was found in cultures during a subsequent 3-week culture period.(ABSTRACT TRUNCATED AT 400 WORDS)
尽管已知神经嵴细胞在其发育过程中对环境线索非常敏感,但最近的证据表明,至少一些亚群在迁移之前可能已确定了特定的分化程序。由于神经嵴由多种细胞组成,这些细胞构成了许多脊椎动物细胞谱系,因此评估特定亚群的特性以及环境对其发育的影响一直很困难。为了解决这个问题,我们用针对一种与高亲和力胆碱摄取相关的75 kDa细胞表面抗原的单克隆抗体(Mabs)标记鸡中脑神经嵴细胞后,通过荧光无流式细胞术分离出了一个纯的亚群。当用这些Mabs和荧光二抗标记鸡中脑神经嵴细胞培养物时,大约5%的细胞为抗原阳性(A+)。分选后,所得培养的中脑神经嵴细胞100%为A+。我们使用的Mabs在体内和体外也标记胚胎鸡和鹌鹑睫状神经节的所有神经元。我们比较了各种细胞培养基对分离出的神经嵴亚群及其来源的异质性鸡中脑神经嵴的影响。A+细胞在含有15%胎牛血清(FBS)和高浓度(10 - 15%)鸡胚提取物的培养基中传代生长,尽管它们保留了基础水平的胆碱乙酰转移酶(ChAT)活性,但没有分化。然而,在鸡血清、高钾(25 mM而非7 mM)以及心脏、虹膜或肺条件培养基中,所有这些都已知可促进睫状神经节神经元的存活和/或胆碱能发育,细胞停止增殖,培养物中的所有细胞在10天内变成“神经元样”。如果使用FBS,在肝脏、脊索或神经管条件培养基中未发现神经元样细胞。当通过补体介导的细胞毒性或在无流式细胞术期间用激光消融A+细胞来去除A+细胞时,所有ChAT活性也被消除,并且在随后的3周培养期内培养物中未发现神经元样细胞或ChAT活性。(摘要截断于400字)
