My usual advice is to calculate a perfect multiplexing level of # sites X read depth and then go much higher. Say you choose to look at 10,000 loci, so the first calculation is 10,000 x 20 = 200,000 reads per sample.

But now assume a 4-fold to 10-fold change in read number from sample to sample. So if the average read number is 200,000 there will be samples at 50,000 reads and samples at 1,000,000 reads.

Because ddRAD has loci defined by two cut sites, each locus has a particular size. If you take a fragment size range of 150-300 bp, the 150 bp fragments will PCR much more than the 300 bp fragments. GC content of the fragment will also affect amplification. So you will have another 10-fold range in locus read depth. Some loci in the low-end samples that got just 50,000 reads will get 1 or 2X read depth instead of the already low 5X.

If you have lots of samples, you will have to make many libraries. So some loci will be in some libraries and not others since the size selection is not perfectly consistent. If you are selecting a wide size range you may just have variable presence of 1000 or fewer loci, but with a tight size range this could be a larger problem.

If your ddRAD fragment has a rare-cutting enzyme and a frequently cutting enzyme, and the population diverse genetically, then you also have to worry about missing data from locus drop-out (see Table 1 of http://www.ncbi.nlm.nih.gov/pubmed/23551379). The issue is that both cut sites, if affected by polymorphism, will drop the locus from the library in that sample. Also, a polymorphism can also create the frequent cut site at the dozen or so "almost cut sites" in a fragment, also removing it from the library.

So if you are wanting to assay 10,000 sites consistently across the population, it is a good idea to accept some missing data in 10% or more of the samples, and you'll want to think about your size selection step and if the genetic diversity of the population will lead to unacceptable levels of drop-out. You can add more loci to partly compensate, but they will also be susceptible to locus drop out, and you may want to avoid 4-cutters or degenerate 5-cutters if the population diversity is very high.

Sounds like a neat project!

Thanks for the quick and helpful reply.

A few further questions ! You say an approximate 10000 loci as an example. Is this a good starting point ? How do I figure the number of loci I should aim for ? Can I get an idea through looking at the existing genome. I also have RNAseq data between some populations under pesticide selection and could maybe estimate SNPs from neutral genes in that data ?

The population diversity is likely to be low; the mites are invasive in regions for only 30 - 100 years and a high percentage of matings are full sibling. This might limit the loci drop-out ?

It sounds like you'll want to assay more than 10,000 sites. If the total population genetic diversity is low, then you'll have a low rate of converting loci to polymorphic SNPs. But it sounds like you might have low diversity within a sample (inbred local population) and unknown total diversity (some inbred populations might be very different from each other). The RNA-Seq data should be a big help in determining what the structure looks like. For a GWAS study you may want more than 10,000 SNPs depending on the size of the blocks of linkage disequilibrium. The shorter they are the more SNPs you'll need. The RNA-Seq data may help there as well since you can find SNPs that are 1kb, 10kb apart and see how often linkage breaks.

If the local population is inbred and you need lots of SNPs and have lots of samples and a limited budget (who doesn't?), then an approach slightly riskier would be to sample lots of loci at low coverage. 10,000 loci at 20X coverage takes the same # of reads as 60,000 at 3X coverage. Just assume the loci are homozygous and that there are very few heterozygous alleles to be missed by using such low coverage anyway. I'm not totally sure how that might affect the GWAS analysis though... again, it probably depends on how inbred they are.

How much DNA can you get from a mite? Do they have endosymbionts like wolbachia? How much of the DNA is mite versus DNA from whatever they eat. We see small insects tend to have a lot more gut-contents DNA in a sample than larger organisms. If you can determine this then you can give more reads to overcome the wasted reads going to other genomes.

I keep forgetting to mention, but if you are in Scotland like your Location says, then some of the most experienced people in using RAD were in the Gene Pool sequencing facility, which is now Edinburgh Genomics. You might check in with them since a local source can be a big help. I'm always happy to discuss projects, though!

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