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首页> 外文期刊>British Journal of Cancer >Pharmacokinetics, binding and distribution of Hoechst 33342 in spheroids and murine tumours
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Pharmacokinetics, binding and distribution of Hoechst 33342 in spheroids and murine tumours

机译:Hoechst 33342在球体和鼠类肿瘤中的药代动力学,结合和分布

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The fluorescent stain Hoechst 33342, when injected i.v. into mice, has an LD50 of 300 micrograms g-1. The stain exits rapidly from the blood, with a half-life of 110 sec following an injection of 10 micrograms g-1, but remains bound within target cells, redistributing with a half-life longer than 2 h. This results in a gradient of drug binding outward from capillaries which can be used to estimate regional perfusion via fluorescence microscopy of frozen tissue sections. For tumour tissues that can be dispersed into single cell suspensions, intracellular Hoeschst 33342 can be quantified by flow cytometry, and cell populations can be selected on the basis of their fluorescence (distance from the vasculature) using a fluorescence-activated cell sorter. Our results in tumours and in spheroids indicate that the rate of stain uptake by different cell subpopulations in situ is much more dependent on stain delivery than on selective uptake. Retention of the stain in spheroids is sufficiently stable to allow cell sorting several hours post-injection. Hoechst 33342 thus appears to have considerable potential as an agent for quantifying tissue perfusion, and for allowing selection of tumour cell subpopulations to assess response to radiation and drugs.
机译:静脉注射荧光染料Hoechst 33342进入小鼠体内的LD50为300微克g-1。污渍从血液中迅速消失,注射10微克g-1后半衰期为110秒,但仍保留在靶细胞内,半衰期超过2小时重新分布。这导致药物从毛细血管向外结合的梯度,该梯度可用于通过冷冻组织切片的荧光显微镜观察区域灌注。对于可以分散到单细胞悬液中的肿瘤组织,可以通过流式细胞术对细胞内的Hoeschst 33342进行定量,并可以使用荧光激活的细胞分选仪根据其荧光(与脉管系统的距离)选择细胞群体。我们在肿瘤和球体中的结果表明,不同细胞亚群原位吸收污渍的速率比选择性吸收更依赖于污渍的传递。球体中污渍的保留足够稳定,可以在注射后数小时进行细胞分选。因此,Hoechst 33342作为定量组织灌注的试剂,并允许选择肿瘤细胞亚群以评估对放射和药物的反应,似乎具有相当大的潜力。

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