What is the variance in the coverage of your genome? For areas that have at least 12 to 15 reads covering 100 base length area, and if you have a single allelic point mutation, you will have a type I error rate of 0.05 and a type II error rate of 0.20. Approximately. This is based on Poisson sampling laws.

This calculation has a TON of assumptions. For example, it assumes that the CNV (copy number variation) is represented in the entire sample, and not a subpopulation of cells. It assumes that the library preparation effects do not treat the different allelic loci in unique ways. For example, there are different types of CNV, and it may place a copy in a GC rich region which can create ligation chemistry biases that result in abnormal quantification (up to 1000-fold off), which will swamp any signal detection of a 2:1 ratio. This separate region may fragment differently and thus may be detected and ligated differently. If the region fragments are smaller for one of the alleles, it may not cluster efficiently on the Illumina, or may not process properly on the Ion Torrent bead populating step with emPCR.

And these are the biases we are aware of that can effect copy abundance measurement.

A PCR-based prep method that captures a variant region of interest can measure allele ratios quite accurately with vary few reads, but requires a priori knowledge of the region of interest.

Sorry, but this is a very difficult area, and based on my experience a 0.5x coverage is quite low sampling to reasonably detect a significant copy number change to any trust-worthy degree.

Regards, -Tom Blomquist

Just to clarify, the above is to detect a 2:1 ratio of alleles.