Preliminary Study on the Nephrotoxicity and its Mechanism of Chuanhuning Injection

XING Wen-min; XU Zhi-lian; LU Hong

doi:10.11653/syfj2013200263

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Preliminary Study on the Nephrotoxicity and its Mechanism of Chuanhuning Injection

更新时间：2024-01-04

- Preliminary Study on the Nephrotoxicity and its Mechanism of Chuanhuning Injection
- Chinese Journal of Experimental Traditional Medical Formulae Vol. 19, Issue 20, Pages: 263-267(2013)
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- DOI：10.11653/syfj2013200263
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- Published：2013
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XING Wen-min, XU Zhi-lian, LU Hong. Preliminary Study on the Nephrotoxicity and its Mechanism of Chuanhuning Injection[J]. Chinese journal of experimental traditional medical formulae, 2013, 19(20): 263-267.
DOI：

XING Wen-min, XU Zhi-lian, LU Hong. Preliminary Study on the Nephrotoxicity and its Mechanism of Chuanhuning Injection[J]. Chinese journal of experimental traditional medical formulae, 2013, 19(20): 263-267. DOI： 10.11653/syfj2013200263.

摘要

目的: 观察穿琥宁注射液(CHN)对小鼠肾毒性作用以及对HK-2细胞活性的影响。方法: 50只ICR小鼠随机分为空白对照组、庆大霉素阳性对照组和CHN 150

1 000

2 000 mg·kg-1剂量组

尾静脉推注

连续7 d

检测体重、肾脏系数、血清尿素氮、肌酐和肾脏组织病理等指标;另采用MTT法测定CHN 干预后HK-2细胞的存活率

荧光染色法(吖啶橙)观察细胞核的形态变化

Annexin V/PI流式细胞术检测细胞凋亡率。结果: 与空白对照组比较

阳性对照组血肌酐明显上升(P<0.05);CHN 2 000 mg·kg-1组肾脏系数明显上升(P<0.05)

血肌酐、尿素氮明显上升(P<0.05)。组织病理学检查显示

CHN 2 000 mg·kg-1组具有肾节段性小管上皮细胞肿胀变性

甚至节段性肾小管变性坏死

伴少量矿物质沉积

部分小管扩张。此外

CHN对HK-2细胞增殖有抑制作用

在0.9~3.5 mmol·L-1浓度和8~48 h时间内CHN对HK-2细胞增殖有抑制作用。荧光染色和Annexin V/PI流式细胞检测结果CHN干预后HK-2细胞可见细胞出现形态不规则、核染色质固缩等细胞凋亡形态学的改变

并且细胞凋亡率随着剂量增加而增大。结论: CHN对小鼠肾脏具有毒性作用

作用可能是通过诱导HK-2细胞凋亡实现。

Abstract

Objective: To observe Chuanhuning injection (CHN)-induced renal toxicity on mice and the cytotoxicity on HK-2 cells. Method: Fifty ICR mice were randomly divided into normal control

positive control group (treated with Gentamycin)

CHN 150

1 000

2 000 mg·kg-1 groups

with 10 mice in each group. Mice in CHN groups were iv given CHN 150

1 000

2 000 mg·kg-1 by tail vein

once daily

for 7 d. The body weight

renal index

serum urea nitrogen and creatinine were assessed

and histopathological changes in renal tissues were detected. The proliferation inhibition of HK-2 cells was determined by MTT assay after different concentration of CHN treatment. The morphological changes of apoptotic cells were observed by the Acridine orange fluorescent staining. Annexin V/PI double staining was utilized to detect the cell apoptosis produced by CHN. Result: Compared with normal control group

serum creatinine in positive control group increased significantly (P<0.05). Compared with positive control group

renal index

serum creatinine and urea nitrogen concentrations in CHN 2 000 mg·kg-1 group increased with significantly statistical difference (P<0.05). Meanwhile

in this group exhibited cloudy swelling even necrosis in proximal convoluted tubules

some minerals deposition in some tubules and extension in section of tubules. CHN suppressed HK-2 cells growth and proliferation within the concentration ranging from 0.9-3.5 mmol·L-1. Fluorescence staining test manifestation series of cell shape changes of apoptosis such as nuclear chromatin condensation. AnnexinV/PI double staining analysis showed that CHN-induced cell apoptosis had significant difference compared with the positive group(P<0.05). Conclusion: CHN may exert toxic actions on kidneys of mice which maybe the outcome of the CHN-induced HK-2 cells apoptosis.

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