I am interested in the data analysis of ChIP-Seq data. I am interested to know how to calculate the following:

1. Log2 Intensity Ratios and what does it mean ? Also, the ratio is between the replicates or between a background and a replicate and how do you calculate the intensity value for each sample?

2. I know how the local regression (lowess) works but why is smoothing needed for ChIP-Seq data. Is it needed to remove the non-specific binding peaks ?

3. What does a genome-wide mean in the ChIP-Seq sample means ?

The questions are based on the Paper that was published in Nature and link of the paper is as follows: http://www.nature.com/nature/journal/v471/n7339/full/nature09725.html.

Any hints or advice will be highly appreciated.

Thanks.

1. The log-ratio is the ratio of the 2 channels in the microarray. See, e.g.: http://en.wikipedia.org/wiki/DNA_microarray#Two-channel_vs._one-channel_detection. Nearly all software packages will do this and other normalization steps for you.
2. Since the probes are often overlapping (http://en.wikipedia.org/wiki/Tiling_array), lowess is used to smooth adjacent / overlapping peaks.
3. ??