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一种新型的器官型脊髓切片氧葡萄糖剥夺模型建立方法。

A novel method for oxygen glucose deprivation model in organotypic spinal cord slices.

机构信息

Department of Neurology, The Second Affiliated Hospital, College of Medicine, Xi'an Jiaotong University, Xi'an, 710004, China.

Department of Ophthalmology, Xi'an No. 3 Hospital, Xi'an, 710018, China.

出版信息

Brain Res Bull. 2017 Oct;135:163-169. doi: 10.1016/j.brainresbull.2017.10.010. Epub 2017 Oct 17.

Abstract

This study aimed to establish a model to closely mimic spinal cord hypoxic-ischemic injury with high production and high reproducibility. Fourteen-day cultured organotypic spinal cord slices were divided into 4 groups: control (Ctrl), oxygen glucose deprived for 30min (OGD 30min), OGD 60min, and OGD 120min. The Ctrl slices were incubated with 1ml propidium iodide (PI) solution (5μg/ml) for 30min. The OGD groups were incubated with 1ml glucose-free DMEM/F12 medium and 5μl PI solution (1mg/ml) for 30min, 60min and 120min, respectively. Positive control slice was fixed by 4% paraformaldehyde for 20min. The culture medium in each group was then collected and the Lactate Dehydrogenase (LDH) level in the medium was tested using Multi-Analyte ELISArray kits. Structure and refraction of the spinal cord slices were observed by light microscope. Fluorescence intensity of PI was examined by fluorescence microscopy and was tested by IPP Software. Morphology of astrocytes was observed by immunofluorescence histochemistry. Caspase 3 and caspase 3 active in different groups were tested by Western blot. In the OGD groups, the refraction of spinal cord slices decreased and the structure was unclear. The changes of refraction and structure in the OGD 120min group were similar to that in the positive control slice. Astrocyte morphology changed significantly. With the increase of OGD time, processes became thick and twisted, and nuclear condensations became more apparent. Obvious changes in morphology were observed in the OGD 60min group, and normal morphology disappeared in the OGD 120min group. Fluorescence intensity of PI increased along with the extension of OGD time. The difference was significant between 30min and 60min, but not significant between 60min and 120min. The intensity at OGD 120min was close to that in the positive control. Compare with the Ctrl group, the OGD groups had significantly higher LDH levels and caspase 3 active/caspase 3 ratios. The values increased with the extension of OGD time and reached peak at 120min. The increase was significant between 30min and 60min, but not significant between 60min and 120min. Organotypic spinal cord slices cultured in glucose-free medium and anaerobic incubator could mimic hypoxia-ischemia of the spinal cord perfectly; 60min could be the best duration for OGD. This technique might be a simple and efficient method to obtain in vitro model for spinal cord hypoxic-ischemic injury in sufficient number and with high quality.

摘要

本研究旨在建立一种能够高度重现脊髓缺氧缺血损伤的模型。将 14 天培养的器官型脊髓切片分为 4 组:对照组(Ctrl)、缺氧葡萄糖剥夺 30min(OGD 30min)、OGD 60min 和 OGD 120min。对照组脊髓切片孵育 1ml 碘化丙啶(PI)溶液(5μg/ml)30min。OGD 组分别孵育 1ml 无葡萄糖 DMEM/F12 培养基和 5μl PI 溶液(1mg/ml)30min、60min 和 120min。阳性对照组切片用 4%多聚甲醛固定 20min。收集每组培养基,使用多分析物 ELISA 试剂盒检测培养基中乳酸脱氢酶(LDH)水平。用光显微镜观察脊髓切片的结构和折射。用荧光显微镜观察 PI 的荧光强度,并使用 IPP 软件进行测试。用免疫荧光组织化学观察星形胶质细胞形态。用 Western blot 检测不同组的 Caspase 3 和活性 Caspase 3。在 OGD 组中,脊髓切片的折射度降低,结构不清晰。OGD 120min 组的折射度和结构变化与阳性对照组切片相似。星形胶质细胞形态发生明显变化。随着 OGD 时间的延长,突起变厚扭曲,核浓缩更加明显。OGD 60min 组可见明显形态改变,OGD 120min 组正常形态消失。PI 荧光强度随 OGD 时间的延长而增加。30min 与 60min 之间差异有统计学意义,但 60min 与 120min 之间差异无统计学意义。OGD 120min 时的强度接近阳性对照组。与对照组相比,OGD 组 LDH 水平和活性 Caspase 3/总 Caspase 3 比值显著升高。随着 OGD 时间的延长而升高,在 120min 时达到峰值。30min 与 60min 之间差异有统计学意义,但 60min 与 120min 之间差异无统计学意义。在无葡萄糖培养基和无氧孵育箱中培养的器官型脊髓切片可完美模拟脊髓缺氧缺血;60min 可能是 OGD 的最佳时间。该技术可能是一种简单高效的方法,可获得足够数量和高质量的脊髓缺氧缺血损伤体外模型。

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