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在小鼠海马体中全身注射红藻氨酸后,AP1 DNA结合的持续增强并不总是与神经元死亡相关。

Sustained potentiation of AP1 DNA binding is not always associated with neuronal death following systemic administration of kainic acid in murine hippocampus.

作者信息

Kitayama T, Ogita K, Yoneda Y

机构信息

Department of Pharmacology, Setsunan University, Hirakata, Osaka, Japan.

出版信息

Neurochem Int. 1999 Dec;35(6):453-62. doi: 10.1016/s0197-0186(99)00088-1.

Abstract

Mice were intraperitoneally injected with kainic acid (KA), followed by dissection of frozen coronal sections and subsequent punching out of the pyramidal and granular cell layers in the hippocampus under a binocular microscope. Systemic administration of KA resulted in marked and sustained potentiation of binding of a radiolabeled double stranded oligonucleotide probe for the nuclear transcription factor activator protein-1 (AP1) in the pyramidal cell layers of the CA1 and CA3 subfields and the granule cell layers of the dentate gyrus 2-18 h later. Morphological evaluation using cresyl violet revealed marked losses of neuronal layers in the pyramidal CA1 and CA3 subfields, but not in the granular dentate gyrus, within 6 weeks after administration. Supershift analysis using antibodies against different Jun and Fos family members differentiated between AP1 DNA binding in hippocampal nuclear extracts obtained 2 and 18 h after the administration of KA. These results suggest that neuronal death may not always follow modulation of de novo synthesis of particular proteins through sustained potentiation of AP1 DNA binding which involves expression of different Jun and Fos family members in response to systemic administration of KA in murine hippocampus.

摘要

给小鼠腹腔注射红藻氨酸(KA),随后解剖冷冻冠状切片,并在双目显微镜下从海马体中冲出锥体细胞层和颗粒细胞层。全身注射KA后2至18小时,在CA1和CA3亚区的锥体细胞层以及齿状回的颗粒细胞层中,放射性标记的双链寡核苷酸探针与核转录因子激活蛋白-1(AP1)的结合显著且持续增强。使用甲酚紫进行的形态学评估显示,给药后6周内,CA1和CA3亚区的锥体细胞层神经元层明显丢失,但齿状回颗粒层未出现这种情况。使用针对不同Jun和Fos家族成员的抗体进行的超迁移分析,区分了KA给药后2小时和18小时从海马体核提取物中获得的AP1 DNA结合情况。这些结果表明,在小鼠海马体中,全身性给予KA后,通过AP1 DNA结合的持续增强(涉及不同Jun和Fos家族成员的表达)来调节特定蛋白质的从头合成,神经元死亡可能并不总是随之发生。

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