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前向散射和侧向散射在流式细胞术检测非整倍体中的相关性。

Relevance of forward scatter and side scatter in aneuploidy detection by flow cytometry.

作者信息

Pétriz J, Tugues D, García-López J

机构信息

Department of Cryobiology and Cell Therapy, Hospital Duran i Reynals, L'Hospitalet del Llobregat, Barcelona, Spain.

出版信息

Anal Cell Pathol. 1996 May;10(3):243-52.

PMID:8798285
Abstract

The study of the nuclear DNA content by flow cytometry (FCM) has been classically accomplished by selecting the nuclear population on the biparametric forward scatter (FS)-DNA fluorescence or FS-DNA fluorescence peak histograms to determine ploidy and DNA index (DI). Different cellular factors such as nuclear morphological heterogeneity of the neoplastic cells, intratumoral variability, histological origin, displasia grade, necrosis, and size of the tumoral piece analyzed constitute important problems in ploidy studies and, consequently, residual or underrepresented clones with different ploidy levels can be masked by populations with a large cell number. In the present report, an alternative methodology is proposed for aneuploidy detection, since populations coinciding with DNA content may be different with respect to morphological criteria. The discrimination of aggregates and background noise by using peak or logarithmic fluorescence signal, and backgating in side scatter (SS)/FS histograms, permits the establishment of specific bounds through complete scatterplot mapping and to distinguish between scarce or minor populations in association with small or abnormal DNA peaks. Moreover, variations in the DNA modal channel value and the peak coefficient of variation value remained unmodified, also maintaining the quality of cytometric measurement data.

摘要

通过流式细胞术(FCM)对核DNA含量进行研究,传统上是通过在双参数前向散射(FS)-DNA荧光或FS-DNA荧光峰直方图上选择核群体来确定倍性和DNA指数(DI)。不同的细胞因素,如肿瘤细胞的核形态异质性、肿瘤内变异性、组织学起源、发育异常等级、坏死以及所分析肿瘤块的大小,在倍性研究中构成了重要问题,因此,具有不同倍性水平的残留或代表性不足的克隆可能会被大量细胞群体所掩盖。在本报告中,提出了一种用于非整倍体检测的替代方法,因为与DNA含量一致的群体在形态学标准方面可能有所不同。通过使用峰值或对数荧光信号以及在侧向散射(SS)/FS直方图中进行反门控来区分聚集体和背景噪声,允许通过完整的散点图映射建立特定界限,并区分与小的或异常DNA峰相关的稀少或次要群体。此外,DNA模态通道值和峰变异系数值的变化保持不变,同时也保持了细胞测量数据的质量。

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