小鼠和大鼠锥体切开术后的神经胶质反应

Leong S.K., Ling E.A., Fan D.P.
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引用次数: 15

摘要

在右侧锥体切除后2 ~ 90天,用灌注法处死成年小鼠和大鼠,观察脑和脊髓内小胶质细胞和星形胶质细胞的反应。用OX-42、OX-18、OX-6对小胶质细胞进行免疫组织化学检测,分别检测补体3型受体和主要组织相容性ⅰ类、ⅱ类抗原的表达。在一些动物中也进行了细胞计数,以确定皮质脊髓束和大脑皮层V层神经元周围可能存在的胶质细胞增殖。部分手术动物给予罗丹明B异硫氰酸酯注射液,观察巨噬细胞/单核细胞是否从血流迁移到反应区。同侧大脑皮层V层神经元细胞体周围的神经胶质反应与假手术动物和正常对照动物的对侧和大脑皮层的神经胶质反应无明显差异。在手术动物的颈椎和腰椎节段,对侧皮质脊髓束的反应性小胶质细胞早在大鼠锥体切除(PP)后2天和小鼠PP后4天出现。小胶质细胞的活化持续到PP 35 d,免疫反应染色逐渐增加,细胞肥大。之后,小胶质细胞免疫反应性减弱,细胞外观恢复正常。定量分析显示,到PP 60天,对侧CST小胶质细胞数量明显增加。在小鼠中,PP 6天,星形胶质细胞肥大,染色更强烈,但数量没有增加。在整个研究期间,大鼠的星形胶质细胞没有明显的变化。罗丹明标记的细胞在病变部位发现,但在大脑皮层的第五层和皮质脊髓束中没有发现。虽然小鼠和大鼠在退行性皮质脊髓束中观察到不同的胶质反应,但两种动物在V层神经元细胞体周围明显缺乏胶质反应。这种缺乏明显的胶质反应不同于以往工作中所证明的外周突出神经元细胞体周围的强烈胶质反应。讨论了这种差异的可能机制以及轴突再生差异的意义。
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Glial Reaction after Pyramidotomy in Mice and Rats

Adult mice and rats were sacrificed by perfusion between 2 and 90 days after right pyramidotomy to study the microglial and astroglial response in the brain and spinal cord. The microglia were detected immunohistochemically with OX-42, OX-18 and OX-6 to assess respectively the expression of complement type 3 receptor, and major histocompatibility class I and class II antigens. Cell counting was also carried out in some animals to determine the possible proliferation of glial cells in the corticospinal tract and around layer V neurons in the cerebral cortex. Some operated animals were given rhodamine B isothiocyanate injection to investigate whether macrophages/monocytes could have migrated from the blood stream to the reactive area. The glial response around the cell bodies of layer V neurons in the ipsilateral cerebral cortex did not display any noticeable difference compared with that of the contralateral side and of the cerebral cortex of the sham-operated and normal control animals. In the cervical and lumbar cord segments of the operated animals, reactive microglial cells in the contralateral corticospinal tract appeared as early as 2 days post pyramidotomy (PP) in rats and 4 days PP in mice. Activation of microglial cells lasted up till 35 days PP, showing gradual increase in immunoreactive staining and hypertrophy. After that, the microglial immunoreactivity subsided and the cells assumed normal appearance by 90 days PP. Quantitative analysis showed a marked increase in the number of microglial cells in the contralateral CST up till 60 days PP. In mice, at 6 days PP, astroglial cells were hypertrophic and more intensely stained but showed no increase in number. No noticeable changes were noted in the astroglia of the rats throughout the period studied. Rhodamine-labelled cells were found at the lesion site, but not in layer V of the cerebral cortex, nor in the corticospinal tract. Though different glial reactions in the degenerating corticospinal tract were noted in mice and rats, there was the same apparent lack of glial reaction around the cell bodies of layer V neurons in the two animal species. Such lack of significant glial response is different from the vigorous glial response around the cell bodies of peripherally projecting neurons demonstrated in previous work. The possible mechanisms for such difference and the implication of the difference in axonal regeneration were discussed.

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