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Toward Automated Analysis of Biofilm Architecture: Bias Caused by Extraneous Confocal Laser Scanning Microscopy Images

机译:走向生物膜结构的自动化分析:外部共聚焦激光扫描显微镜图像引起的偏差

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摘要

An increasing number of studies utilize confocal laser scanning microscopy (CLSM) for in situ visualization of biofilms and rely on the use of image analysis programs to extract quantitative descriptors of architecture. Recently, designed programs have begun incorporating procedures to automatically determine threshold values for three-dimensional CLSM image stacks. We have found that the automated threshold calculation is biased when a stack contains images lacking pixels of biological significance. Consequently, we have created the novel program Auto PHLIP-ML to resolve this bias by iteratively excluding extraneous images based on their area coverage of biomass. A procedure was developed to identify the optimal percent area coverage value used for extraneous image removal (PACVEIR). The optimal PACVEIR was defined to occur when the standard deviation of mean thickness, determined from replicate image stacks, was at a maximum, because it more accurately reflected inherent structural variation. Ten monoculture biofilms of either Ralstonia eutropha JMP228n::gfp or Acinetobacter sp. strain BD413 were tested to verify the routine. All biofilms exhibited an optimal PACVEIR between 0 and 1%. Prior to the exclusion of extraneous images, JMP228n::gfp appeared to develop more homogeneous biofilms than BD413. However, after the removal of extraneous images, JMP228n::gfp biofilms were found to form more heterogeneous biofilms. Similarly, JMP228n::gfp biofilms grown on glass surfaces vis-à-vis polyethylene membranes produced significantly different architectures after extraneous images had been removed but not when such images were included in threshold calculations. This study shows that the failure to remove extraneous images skewed a seemingly objective analysis of biofilm architecture and significantly altered statistically derived conclusions.
机译:越来越多的研究利用共聚焦激光扫描显微镜(CLSM)对生物膜进行原位可视化,并依靠图像分析程序来提取建筑的定量描述。最近,已设计的程序已开始合并自动为三维CLSM图像堆栈确定阈值的过程。我们发现,当堆栈中包含缺乏生物学意义的像素的图像时,自动阈值计算会产生偏差。因此,我们创建了新颖的程序Auto PHLIP-ML来解决此偏差,方法是根据其生物量的面积覆盖范围反复排除无关图像。开发了一种程序来确定用于去除多余图像(PACVEIR)的最佳区域覆盖率百分比值。最佳PACVEIR定义为当从复制图像堆栈确定的平均厚度的标准偏差最大时发生,因为它可以更准确地反映固有的结构变化。 Ralstonia eutropha JMP228n :: gfp或不动杆菌属的十个单培养生物膜。测试了BD413菌株以验证该程序。所有生物膜均表现出0%至1%的最佳PACVEIR。在排除无关图像之前,JMP228n :: gfp似乎比BD413形成了更多均匀的生物膜。然而,去除无关的图像后,发现JMP228n :: gfp生物膜形成了更多的异质生物膜。同样,在玻璃表面上相对于聚乙烯膜生长的JMP228n :: gfp生物膜在去除无关图像后产生了显着不同的体系结构,但是当阈值计算中包括了此类图像时则没有。这项研究表明,未能去除多余的图像使生物膜结构的看似客观的分析失真,并大大改变了统计得出的结论。

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