头孢立啶在正常血糖和糖尿病大鼠肾片中的体外毒性和蓄积

Monica Valentovic, John G. Ball, Bethany A. Rogers, M.Kathleen Meadows, R.Christopher Harmon , Joshua Moles
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引用次数: 0

摘要

先前的研究表明,头孢啶在糖尿病大鼠模型中的肾毒性降低。接下来的研究检查了正常血糖和糖尿病Fischer 344大鼠肾片中的玻璃脑吖啶毒性。急性腹腔注射链脲佐菌素35 mg/kg诱导糖尿病。取血糖正常和糖尿病动物肾皮质切片。组织暴露于0-5 mmcephaloridine 15-120分钟。暴露于2-5 mmcephaloridine 60-120分钟的所有组中,丙酮酸定向糖异生都减少。只有血糖正常组在4-5 mmcephaloridine存在120分钟时,乳酸脱氢酶(LDH)渗漏明显。在任何浓度的cephaloridine下,糖尿病组织中LDH渗漏均未增加。在暴露于头孢啶30-120分钟的肾皮质切片中,比较了总谷胱甘肽水平。血糖正常和糖尿病组织中谷胱甘肽的基线值是相似的,这表明降低毒性的机制不是由于糖尿病组织中较高的谷胱甘肽水平。在血糖正常的组织中,总谷胱甘肽水平比用5毫头孢啶孵育的糖尿病组织降低得更快。头孢利啶积累比较表明,0-2 mmcephaloridine孵育时,糖尿病组织积累的头孢利啶少于正常血糖组。然而,在4-5 mmcephaloridine体外培养后,正常血糖组和糖尿病组的肾片积累相似。这些结果表明,糖尿病组织中玻璃脑嘧啶毒性降低的机制不能局限于积累的差异,而必须包括一种未知的细胞成分。
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Cephaloridinein VitroToxicity and Accumulation in Renal Slices from Normoglycemic and Diabetic Rats

Previous work has shown a reduction in cephaloridine nephrotoxicity in a diabetic rat model. The following studies examinedin vitrocephaloridine toxicity in renal slices from normoglycemic and diabetic Fischer 344 rats. Diabetes was induced by acute intraperitoneal injection of 35 mg/kg streptozotocin. Renal cortical slices were isolated from normoglycemic and diabetic animals. Tissues were exposed to 0–5 mmcephaloridine for 15–120 min. Pyruvate-directed gluconeogenesis was diminished in all groups exposed to 2–5 mmcephaloridine for 60–120 min. Leakage of lactate dehydrogenase (LDH) was apparent only in the normoglycemic group in the presence of 4–5 mmcephaloridine for 120 min. LDH leakagewas notincreased at any cephaloridine concentration in the diabetic tissue. Total glutathione levels were compared in renal cortical slices exposed to cephaloridine for 30–120 min. Baseline values for glutathione were comparable between normoglycemic and diabetic tissue suggesting that the mechanism for reduced toxicity was not due to higher glutathione levels in diabetic tissue. Total glutathione levels were diminished more rapidly in normoglycemic than diabetic tissue by incubation with 5 mmcephaloridine. Comparison of cephaloridine accumulation indicated that diabetic tissue accumulated less cephaloridine than the normoglycemic group when tissues were incubated with 0–2 mmcephaloridine. However, renal slice accumulation was similar between normoglycemic and diabetic groups followingin vitroincubation with 4–5 mmcephaloridine. These results suggest that the mechanism for reducedin vitrocephaloridine toxicity in diabetic tissue cannot be limited to differences in accumulation and must include an unidentified cellular component.

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