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2,2'-偶氮二(2-脒基丙烷)二盐酸盐增强超声诱导对单核细胞U937细胞的杀伤作用。

Ultrasound-induced killing of monocytic U937 cells enhanced by 2,2'-azobis(2-amidinopropane) dihydrochloride.

作者信息

Feril Loreto B, Tsuda Yuko, Kondo Takashi, Zhao Qing-Li, Ogawa Ryohei, Cui Zheng-Guo, Tsukada Kazuhiro, Riesz Peter

机构信息

Department of Radiological Sciences, Toyama Medical and Pharmaceutical University, Toyama 930-0194, Japan.

出版信息

Cancer Sci. 2004 Feb;95(2):181-5. doi: 10.1111/j.1349-7006.2004.tb03201.x.

Abstract

To determine the effect of 2,2'-azobis(2-amidinopropane) dihydrochloride (AAPH) on ultrasound (US)-induced cell killing, human monocytic leukemia cells (U937) were incubated at various temperatures (25.0, 37.0 and 40.0 degrees C) for 1 min in air-saturated phosphate-buffered solution (PBS) containing 50 mM AAPH before exposure to nonthermal 1 MHz US for 1 min at an intensity of 2.0 W/cm(2). Cell viability was determined by means of the Trypan blue dye exclusion test immediately after sonication. Apoptosis was measured after 6-h incubation post-sonication by flow cytometry. Free radicals generated by AAPH, a temperature-dependent free radical generator, or US or both were also investigated using electron paramagnetic resonance (EPR) spin trapping. The results showed that US-induced cell lysis and apoptosis were enhanced in the presence of AAPH regardless of the temperature at the time of sonication. At 40.0 degrees C, US alone induced increased cell killing, while AAPH alone is capable of inducing significant but minimal apoptosis at this temperature. Although free radicals were increased in the combined treatment, this increase did not correlate well with cell killing. The mechanism of enhancement points to the increased uptake of the agent during sonication rather than potentiation by AAPH. These findings suggest the clinical potential of temperature-dependent free radical generators in cancer therapy with therapeutic US.

摘要

为了确定2,2'-偶氮二异丁脒二盐酸盐(AAPH)对超声(US)诱导的细胞杀伤作用,在暴露于强度为2.0W/cm²的1MHz非热超声1分钟之前,将人单核细胞白血病细胞(U937)在含有50mM AAPH的空气饱和磷酸盐缓冲溶液(PBS)中于不同温度(25.0、37.0和40.0℃)孵育1分钟。超声处理后立即通过台盼蓝染料排除试验测定细胞活力。超声处理后孵育6小时后通过流式细胞术测量细胞凋亡。还使用电子顺磁共振(EPR)自旋捕获技术研究了由AAPH(一种温度依赖性自由基产生剂)、超声或两者产生的自由基。结果表明,无论超声处理时的温度如何,在AAPH存在的情况下,超声诱导的细胞裂解和凋亡均增强。在40.0℃时,单独超声诱导细胞杀伤增加,而单独的AAPH在此温度下能够诱导显著但最小程度的细胞凋亡。尽管联合处理中自由基增加,但这种增加与细胞杀伤的相关性不佳。增强机制表明超声处理期间药物摄取增加,而非AAPH的增效作用。这些发现提示温度依赖性自由基产生剂在超声治疗癌症中的临床潜力。

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