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Once the .idat files are imported, you will be facing the Scatter Plot. To move forward with the tutorial, switch to the Analysis tab and take a look at the top level (i.e. initial) spreadsheet (Figure 1). Samples identifiers are the names of the .idat files as shown by the Sample ID column while all the remaining columns are the array probes.

 

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SubtitleTextSpreadsheet after .idat file import: samples on rows (Sample IDs are based on file names), probes on columns, cell values are functionally normalized beta values (default settings)
AnchorNametop level spreadsheet

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As discussed in the previous chapter, the values in the cells are normalized β-values, which correspond to the percentage of methylation at each site and are calculated as the ratio of methylated probe intensity over the overall intensity at each site (the overall intensity is the sum of methylated and unmethylated probe intensities). An alternative metric for measurement of methlyation levels are M-values. β-values can be easily converted to M-values using the following equation:

M-value = log2( β / (1 - β))

Here's the interpretation: a M-value close to 0 indicates a similar intensity between the methylated and unmethylated probes, which means the CpG site is about half-methylated. Positive M-values mean that more molecules are methylated than unmethylated, while negative M-values mean that more molecules are unmethylated than methylated.  As discussed by Du and colleagues, the β-value has a more intuitive biological interpretation, but the M-value is more statistically valid for the differential analysis of methylation levels.

Therefore, the differential methylation analysis of the tutorial data will be performed on the M-values; select Convert Beta Value to M Value from the workflow. Note that the original data (β-values) will be overwritten.

 

 

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