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短链脂肪酸对培养的原代尿路上皮细胞的影响:对肠膀胱扩大术中膀胱内应用的意义。

Effects of short-chain fatty acids on primary urothelial cells in culture: implications for intravesical use in enterocystoplasties.

作者信息

Solomon L Z, Jennings A M, Sharpe P, Cooper A J, Malone P S

机构信息

Department of Paediatric Urology, Southampton University Hospitals NHS Trust, England.

出版信息

J Lab Clin Med. 1998 Oct;132(4):279-83. doi: 10.1016/s0022-2143(98)90040-3.

Abstract

The presence of inflammatory changes and mucopus production in an enterocystoplasty may be similar to the condition of diversion colitis and starvation diarrhea caused by a lack of luminal short-chain fatty acids (SCFAs). We postulate a therapeutic role for intravesical SCFA. Because this treatment will also contact the urothelium, we have assessed the effect on cellular proliferation by utilizing primary urothelial cells in culture. Primary urothelial cells were grown from biopsy samples of normal urothelium obtained intraoperatively. A cocktail of SCFA used in the treatment of diversion colitis was incubated with these cells for time intervals ranging from 30 minutes to 72 hours at drug concentrations ranging from 0.04 to 20 mmol/L butyrate equivalent (BE). The 3-(4,5-dimethylthiazol-2-yl)-2,5-diphenyltetrazolium bromide (MTT) assay was used to measure the residual viable biomass to assess growth inhibition. These experiments were repeated on cells grown on matrigel substrate. The human urothelial cancer line RT112 was likewise exposed to SCFAs to assess selectivity between primary and transformed cells. Primary urothelial cells in culture undergo growth inhibition when exposed to SCFAs. The concentration of SCFAs required to reduce the general biomass by 50% or more (IC> or =50) was 20 mmol/L BE when exposure was for 2 hours or less. When drug exposure was prolonged for 72 hours, the IC> or =50 was 2.5 mmol/L BE. Cells grown on matrigel had their growth similarly inhibited. The IC > or = 50 for the RT112 cell line was 2.5 mmol/L BE after 72 hours of drug incubation. Primary urothelial cells in culture undergo a time- and dose-dependent growth inhibition when exposed to SCFAs. This inhibition is particularly apparent at the higher doses similar to those in use in clinical practice. Cells grown on a matrigel substrate suffer growth attenuation similar to that affecting cells grown on polystyrene plates. In vivo assessment in a rodent intravesical model is advisable before considering instillations in patients.

摘要

肠膀胱扩大术中出现的炎症变化和黏液分泌可能类似于因缺乏肠腔内短链脂肪酸(SCFAs)引起的改道性结肠炎和饥饿性腹泻的情况。我们推测膀胱内注入SCFAs具有治疗作用。由于这种治疗也会接触尿路上皮,我们利用培养的原代尿路上皮细胞评估了其对细胞增殖的影响。原代尿路上皮细胞从术中获取的正常尿路上皮活检样本中培养而来。用于治疗改道性结肠炎的SCFAs混合物与这些细胞在0.04至20 mmol/L丁酸当量(BE)的药物浓度下孵育30分钟至72小时。采用3-(4,5-二甲基噻唑-2-基)-2,5-二苯基四氮唑溴盐(MTT)法测量残余活细胞量以评估生长抑制情况。在基质胶上生长的细胞重复进行了这些实验。人尿路上皮癌细胞系RT112同样暴露于SCFAs中,以评估原代细胞和转化细胞之间的选择性。培养的原代尿路上皮细胞暴露于SCFAs时会受到生长抑制。暴露2小时或更短时间时,使总体细胞量减少50%或更多(IC≥50)所需的SCFAs浓度为20 mmol/L BE。当药物暴露延长至72小时时,IC≥50为2.5 mmol/L BE。在基质胶上生长的细胞其生长同样受到抑制。药物孵育72小时后,RT112细胞系的IC≥50为2.5 mmol/L BE。培养的原代尿路上皮细胞暴露于SCFAs时会经历时间和剂量依赖性的生长抑制。这种抑制在与临床实践中使用的较高剂量相似时尤为明显。在基质胶上生长的细胞生长减弱情况与在聚苯乙烯板上生长的细胞相似。在考虑对患者进行灌注之前,建议在啮齿动物膀胱内模型中进行体内评估。

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