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正常兔角膜前后角膜细胞密度的定量评估。

Quantitative assessment of anteroposterior keratocyte density in the normal rabbit cornea.

作者信息

Petroll W M, Boettcher K, Barry P, Cavanagh H D, Jester J V

机构信息

Department of Ophthalmology, University of Texas Southwestern Medical Center, Dallas 75235-9057.

出版信息

Cornea. 1995 Jan;14(1):3-9.

PMID:7712733
Abstract

The anteroposterior keratocyte density distribution in the rabbit cornea was measured. Unsectioned tissue blocks from the central cornea of five rabbits were stained with propidium iodide and imaged using a Leica laser scanning confocal microscope. A z-series of images was acquired confocal microscope. A z-series of images was acquired in each sample, from anterior to posterior stroma in either 3- or 8-microns steps. Software was developed to allow interactive marking of the keratocyte nuclei within each section of the z-series and for calculating cell density. For convenience, cell density was expressed as the number of cells per corneal volume element (CVE), where CVE is a newly defined volume unit with x, y, and z dimensions of 250, 250, and 10 microns, respectively. The calculated keratocyte density was 20.2 +/- 1.0 cells/CVE (n = 5), which is equivalent to 32,360 +/- 1,660 cells/mm3. The greatest density was underneath the epithelium (26.3 +/- 2.5 cells/CVE), the density then decreased linearly with depth to 15.2 +/- 1.4 cells/CVE; there was a slight increase in density pre-Descemets membrane to 18.5 +/- 3.5 cells/CVE. A 30% decrease in cell density over the entire anteroposterior stromal thickness was observed. To facilitate statistical analysis, the cell density was averaged over 5% thickness intervals from anterior to posterior cornea. A significant difference in mean cell density of these intervals was found (ANOVA, n = 20, p < 0.01). To further assess the density distribution, linear regression analysis was performed. A significant correlation was found between keratocyte density and stromal depth (R = -0.94, n = 20, p < 0.05).(ABSTRACT TRUNCATED AT 250 WORDS)

摘要

测量了兔角膜前后方向的角膜细胞密度分布。取自五只兔子中央角膜的未切片组织块用碘化丙啶染色,并使用徕卡激光扫描共聚焦显微镜成像。在共聚焦显微镜下采集每个样本从前到后基质的一系列z轴图像,步长为3微米或8微米。开发了软件以允许对z轴系列每个切片中的角膜细胞核进行交互式标记并计算细胞密度。为方便起见,细胞密度表示为每角膜体积单元(CVE)的细胞数,其中CVE是一个新定义的体积单位,其x、y和z维度分别为250微米、250微米和10微米。计算出的角膜细胞密度为20.2±1.0个细胞/CVE(n = 5),相当于32360±1660个细胞/mm³。最大密度位于上皮下方(26.3±2.5个细胞/CVE),然后密度随深度呈线性下降至15.2±1.4个细胞/CVE;在Descemet膜前密度略有增加至18.5±3.5个细胞/CVE。观察到整个前后基质厚度的细胞密度下降了30%。为便于统计分析,从角膜前到后以5%厚度间隔对细胞密度进行平均。发现这些间隔的平均细胞密度存在显著差异(方差分析,n = 20,p < 0.01)。为进一步评估密度分布,进行了线性回归分析。发现角膜细胞密度与基质深度之间存在显著相关性(R = -0.94,n = 20,p < 0.05)。(摘要截断于250字)

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