Peeters M C, Schutte B, Lenders M H, Hekking J W, Drukker J, Van Straaten H W
Department of Anatomy and Embryology, University of Maastricht, The Netherlands.
Dev Dyn. 1998 Apr;211(4):382-9. doi: 10.1002/(SICI)1097-0177(199804)211:4<382::AID-AJA9>3.0.CO;2-D.
In the mouse mutant curly tail, the phenotypes spina bifida and curled tail result from a delay in closure of the posterior neuropore (PNP). At the developmental stage when this delay can first be recognized, the caudal region of the embryo demonstrates a transiently enhanced curvature of the body axis which likely inhibits elevation, convergence, and fusion of the neural folds. The enhanced curvature is thought to be the result of a decreased proliferation in the ventrally located gut endoderm and notochord, together with a normal proliferation of the overlying neuroepithelium of the PNP. However, the proliferation defect and the enhanced curvature were originally demonstrated at the same developmental stage, while it is expected that reduced proliferation should precede enhanced curvature and delayed PNP closure. The caudal region originates from the tail bud and we therefore propose that the enhanced curvature is induced by a disturbed dorso-ventral proliferation pattern in the tail bud. Using flow cytometry, proliferation patterns were determined separately for the dorsal and ventral halves of the tail bud of curly tail and of control embryos as well as of recombinant embryos having the curly tail phenotype with a genetic background which is matched to the BALB/c control strain. In general, it appeared that about half of the cell cycle duration in tail bud cells was occupied by S phase, about 40% by G0/G1 and the rest by G2/M. For the control embryos, no dorso-ventral differences in relative phase duration were demonstrated. However, curly tail and recombinant embryos at the 21-25 somite stage, prior to the onset of enhanced curvature, exhibited ventrally a higher proportion of G0/G1 phase cells than dorsally, and a complementary relationship for S phase cells. We interpret these observations as indicating a prolonged G1 phase at the ventral side of the tail bud, resulting in a prolongation of the cell cycle and thus a decreased proliferation. In 26-30 somite stage embryos, prior to the normalization of curvature in curly tail embryos, the dorso-ventral proliferation balance was re-established. We conclude that a reduced proliferation in the ventral part of the tail bud of the curly tail embryo precedes both the onset of enhanced curvature and the previously observed reduction in proliferation of the hindgut and notochord, and is a likely candidate for an early event in the pathogenetic sequence leading to the curly tail phenotype.
在小鼠突变体卷尾中,脊柱裂和卷尾表型是由后神经孔(PNP)闭合延迟导致的。在首次识别出这种延迟的发育阶段,胚胎的尾部区域表现出体轴的短暂增强弯曲,这可能会抑制神经褶的抬高、汇聚和融合。这种增强的弯曲被认为是腹侧肠道内胚层和脊索增殖减少的结果,同时PNP上方的神经上皮正常增殖。然而,增殖缺陷和增强的弯曲最初是在同一发育阶段被证实的,而预期增殖减少应先于弯曲增强和PNP闭合延迟。尾部区域起源于尾芽,因此我们提出增强的弯曲是由尾芽中背腹增殖模式紊乱诱导的。使用流式细胞术,分别确定了卷尾胚胎和对照胚胎以及具有与BALB/c对照品系匹配的遗传背景的具有卷尾表型的重组胚胎尾芽背侧和腹侧的增殖模式。总体而言,似乎尾芽细胞中约一半的细胞周期持续时间由S期占据,约40%由G0/G1期占据,其余由G2/M期占据。对于对照胚胎,未显示相对相持续时间的背腹差异。然而,在21 - 25体节阶段、弯曲增强开始之前的卷尾和重组胚胎,腹侧的G0/G1期细胞比例高于背侧,S期细胞呈互补关系。我们将这些观察结果解释为表明尾芽腹侧的G1期延长,导致细胞周期延长,从而增殖减少。在26 - 30体节阶段的胚胎中,在卷尾胚胎弯曲正常化之前,背腹增殖平衡得以重建。我们得出结论,卷尾胚胎尾芽腹侧增殖减少先于弯曲增强的开始以及先前观察到的后肠和脊索增殖减少,并且是导致卷尾表型的发病序列中早期事件的可能候选因素。
