Maier S E, West J R
Human Anatomy and Medical Neurobiology, The Texas A&M University, System Health Science Center, College Station, TX 77843-1114, USA.
Alcohol. 2001 Jan;23(1):49-57. doi: 10.1016/s0741-8329(00)00133-6.
Women who abuse alcohol during pregnancy may deliver offspring who could be diagnosed with fetal alcohol syndrome (FAS) or a less severe deficit involving cognitive and behavioral disorders. The severity of the deficits may involve the interaction of several known risk factors, such as alcohol consumption pattern or duration, the timing of alcohol consumption relative to critical windows of vulnerability, or the inherent differential vulnerability among the various brain regions to alcohol-induced brain injury. In this study, we explore the vulnerability of the different brain regions by making cell counts from multiple brain regions. Specifically, we used stereological cell-counting techniques to estimate the total cell numbers in the cerebellum (Purkinje and granule cells), olfactory bulb (mitral and granule cells), hippocampus (CA1 and CA3 cells), and dentate gyrus (granule cells). Groups of timed-pregnant Sprague-Dawley rats were assigned to one of five treatments: alcohol by intragastric intubation (2.25, 4.5, or 6.5 g/kg/day), nutritional control [pairfed and intubated=Pairfed) and intubated], and normal control (Chow). Treatments began on embryonic day 1 (E1) and continued through E20. On E33 (usually postnatal day 10), all offspring were perfused intracardially with saline followed by fixatives. Representative forebrains, cerebella, and olfactory bulb from each group were processed for cell counting. The optical dissector was used to obtain cell densities, while Cavalieri's principle was used to calculate the reference volume. The product of density and volume gave unbiased estimates of the total neuronal number within each brain region. Overall peak BACs (regardless of sampling day) for the three alcohol groups averaged 136, 290, and 422 mg/dl for the 2.25-, 4.5-, and 6.5-g/kg groups, respectively. The total number of cerebellar Purkinje cells was reduced in the 6.5-g/kg group relative to controls, while the total number of olfactory bulb mitral cells and hippocampal CA1 and CA3 pyramidal cells from all alcohol-treated groups was not different from controls. Total numbers of granule neurons were reduced in the cerebellum and olfactory bulb of offspring exposed to 4.5 or 6.5 g/kg/day, but granule cell numbers in the dentate gyrus were not affected by the prenatal alcohol treatment. Taken together with previous findings, these data demonstrate that prenatal alcohol exposure results in regional vulnerability of various brain structures and underscores the variability of deleterious effects of alcohol on brain development.
孕期酗酒的女性所分娩的后代可能会被诊断为胎儿酒精综合征(FAS)或患有涉及认知和行为障碍的不太严重的缺陷。这些缺陷的严重程度可能涉及几个已知风险因素的相互作用,如饮酒模式或持续时间、饮酒时间相对于关键易损期的关系,或不同脑区对酒精诱导脑损伤的固有差异易损性。在本研究中,我们通过对多个脑区进行细胞计数来探究不同脑区的易损性。具体而言,我们使用体视学细胞计数技术来估计小脑(浦肯野细胞和颗粒细胞)、嗅球(二尖瓣细胞和颗粒细胞)、海马体(CA1和CA3细胞)以及齿状回(颗粒细胞)中的细胞总数。将定时怀孕的斯普拉格-道利大鼠分组,分别给予五种处理之一:经胃插管给予酒精(2.25、4.5或6.5克/千克/天)、营养对照(配对喂食并插管=配对喂食组并插管)以及正常对照(普通饲料)。处理从胚胎第1天(E1)开始,持续至E20。在E33(通常为出生后第10天),所有后代经心脏灌注生理盐水,随后灌注固定剂。对每组的代表性前脑、小脑和嗅球进行细胞计数处理。使用光学分割器获取细胞密度,同时运用卡瓦列里原理计算参考体积。密度与体积的乘积得出每个脑区内神经元总数的无偏估计值。三个酒精组的总体峰值血液酒精浓度(无论采样日如何),2.25克/千克组、4.5克/千克组和6.5克/千克组分别平均为136、290和422毫克/分升。与对照组相比,6.5克/千克组的小脑浦肯野细胞总数减少,而所有酒精处理组的嗅球二尖瓣细胞以及海马体CA1和CA3锥体细胞总数与对照组无差异。暴露于4.5或6.5克/千克/天酒精的后代,其小脑和嗅球中的颗粒神经元总数减少,但产前酒精处理对齿状回中的颗粒细胞数量没有影响。结合先前的研究结果,这些数据表明产前酒精暴露会导致各种脑结构出现区域易损性,并强调了酒精对脑发育有害影响的变异性。
