Noraberg Jens
NeuroScreen ApS, Anatomy and Neurobiology, University of Southern Denmark, Winslowparken 21, 5000 Odense, Denmark.
Altern Lab Anim. 2004 Oct;32(4):329-37. doi: 10.1177/026119290403200403.
This paper reviews the current state of the use of organotypic brain slice cultures for neurotoxicological and neuropharmacological screening and mechanistic studies, as exemplified by excitotoxin application. At present, no in vitro systems have been approved by the regulatory authorities for neurotoxicity testing. For the evaluation of the slice culture method, organotypic hippocampal slice cultures were exposed to toxic doses of the excitotoxins, glutamate, N-methyl-D-aspartate (NMDA), kainic acid and 2-amino-3-hydroxy-5-methyl-4-isoxazole propionate (AMPA), and the glial toxin, DL-alpha-aminoadipic acid (DLAAA). Neuronal cell death was quantified by propidium iodide (PI) uptake, and visualised by Fluoro-Jade (FJ) staining. General cell death was monitored by lactate dehydrogenase (LDH) release into the culture medium. EC50 values for the different compounds, based on PI uptake after exposure for 48 hours in entire cultures, were: glutamate, 3.5 mM; DL-AAA, 2.3 mM; kainic acid, 13 microM; NMDA, 11 microM; and AMPA, 3.7 microM. In the slice cultures, the hippocampal subfields displayed the same differences in vulnerability as those observed in vivo. When subfield analysis was performed on the cultures, the CA1 subfield was most susceptible to glutamate, NMDA and AMPA, while CA3 was most susceptible to kainic acid. The amount of LDH release for DL-AAA was about four times that of L-glutamate, in accordance with the additional toxic effect on glial cells, which was also found by confocal microscopy to stain for FJ. In conclusion, it was found that organotypic brain slice culture, combined with standardised protocols and quantifiable markers, such as PI and FJ staining, is a relevant and feasible in vitro system for neurotoxicity testing. Considering the amount and quality of the available published data, it is recommended that the brain slice culture method could be subjected to pre-validation and formal validation for inclusion in a tiered in vitro neurotoxicity testing scheme to supplement and replace conventional animal tests.
本文回顾了器官型脑片培养在神经毒理学和神经药理学筛选及机制研究中的应用现状,以兴奋性毒素应用为例。目前,尚无体外系统获得监管机构批准用于神经毒性测试。为评估脑片培养方法,将器官型海马脑片培养物暴露于毒性剂量的兴奋性毒素(谷氨酸、N-甲基-D-天冬氨酸(NMDA)、海人酸和2-氨基-3-羟基-5-甲基-4-异恶唑丙酸(AMPA))以及胶质毒素DL-α-氨基己二酸(DLAAA)。通过碘化丙啶(PI)摄取对神经元细胞死亡进行定量,并通过荧光玉(FJ)染色进行可视化。通过监测乳酸脱氢酶(LDH)释放到培养基中来监测一般细胞死亡。基于在整个培养物中暴露48小时后的PI摄取,不同化合物的半数有效浓度(EC50)值为:谷氨酸3.5 mM;DL-AAA 2.3 mM;海人酸13 μM;NMDA 11 μM;AMPA 3.7 μM。在脑片培养物中,海马亚区显示出与体内观察到的相同的易损性差异。对培养物进行亚区分析时,CA1亚区对谷氨酸、NMDA和AMPA最敏感,而CA3对海人酸最敏感。DL-AAA的LDH释放量约为L-谷氨酸的四倍,这与对胶质细胞的额外毒性作用一致,共聚焦显微镜检查也发现其对FJ染色。总之,发现器官型脑片培养结合标准化方案和可量化标记物(如PI和FJ染色)是一种用于神经毒性测试的相关且可行的体外系统。考虑到现有已发表数据的数量和质量,建议对脑片培养方法进行预验证和正式验证,以纳入分层体外神经毒性测试方案,以补充和替代传统动物试验。
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