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A new approach to intensity-dependent normalization of two-channel microarrays

机译:强度依赖的双通道微阵列归一化的新方法

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A two-channel microarray measures the relative expression levels of thousands of genes from a pair of biological samples. In order to reliably compare gene expression levels between and within arrays, it is necessary to remove systematic errors that distort the biological signal of interest. The standard for accomplishing this is smoothing "MA-plots" to remove intensity-dependent dye bias and array-specific effects. However, MA methods require strong assumptions, which limit their general applicability. We review these assumptions and derive several practical scenarios in which they fail. The "dye-swap" normalization method has been much less frequently used because it requires two arrays per pair of samples. We show that a dye-swap is accurate under general assumptions, even under intensity-dependent dye bias, and that a dye-swap removes dye bias from a single pair of samples in general. Based on a flexible model of the relationship between mRNA amount and single-channel fluorescence intensity, we demonstrate the general applicability of a dye-swap approach. We then propose a common array dye-swap (CADS) method for the normalization of two-channel microarrays. We show that CADS removes both dye bias and array-specific effects, and preserves the true differential expression signal for every gene under the assumptions of the model.
机译:两通道微阵列可测量一对生物学样品中数千个基因的相对表达水平。为了可靠地比较阵列之间和阵列内的基因表达水平,有必要消除使感兴趣的生物信号失真的系统错误。实现此目的的标准是平滑“ MA-plots”以消除强度相关的染料偏差和特定于阵列的效果。但是,MA方法需要强有力的假设,这限制了它们的普遍适用性。我们回顾了这些假设,并得出了一些失败的实际情况。 “染料交换”归一化方法使用的频率要低得多,因为它每对样本需要两个阵列。我们显示,在一般假设下,即使在强度依赖的染料偏差下,染料交换也是准确的,并且染料交换通常可从一对样品中去除染料偏差。基于mRNA量和单通道荧光强度之间关系的灵活模型,我们证明了染料交换方法的普遍适用性。然后,我们提出了一种用于两通道微阵列归一化的通用阵列染料交换(CADS)方法。我们表明,CADS消除了染料偏差和阵列特异性效应,并在模型假设下为每个基因保留了真正的差异表达信号。

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