This post is by Josh Schraiber on his paper (along with coauthors): Schraiber et al. Inferring non-neutral regulatory change in pathways from transcriptional profiling data arXived here.

We’ve known for a long time now that gene sequence alone does not determine phenotype. From the trivial example of differentiated cell types (which all have the same DNA) to now-common examples where species adapt to their environment by changing something other than protein-coding sequence, it’s clear that the expression level of a gene plays just as important a role in phenotypic development as does its sequence. Despite this fact, we still lack the kinds of tools that are widely available for detecting non-neutral evolution at the level of gene expression (in packages like PAML). Part of this problem lies in a fundamental lack of power. A single gene may have hundreds of sites, and the patterns that occur at all of those sites give us plenty of information to learn about accelerated substation rates and the like. But a gene (in a given environment) has just one expression level, so the sample size is often small and power is reduced.

This same problem occurs, of course, in phylogenetic studies of quantitative characters at the organismal level. The difference is that in those cases, researchers typically have access to tens, if not hundreds, of species with good quality measurements. Unfortunately, transcriptome-wide gene expression data can be difficult and costly to collect, so large-scale studies are few and far between.

Instead of trying to leverage large collections of species, we sought to utilize one of the benefits of transcriptome-wide profiles: data from lots and lots of genes. A common practice in molecular evolution is to run tests for selection on a gene-by-gene basis and then look for functional groups that are overrepresented (e.g. Gene Ontology enrichment). We turned that around and instead started with a priori defined gene groups (in our case, from Gene Ontology), looking to detect signal for a history of lineage-specific gene expression evolution, by jointly analyzing all the genes in a group simultaneously.

Doing this would potentially run into a problem of overfitting: should we try to fit a separate rate of evolution for each gene in the group? Instead, we borrowed a page from Ziheng Yang’s book and assumed that the rate of evolution across genes was inverse-gamma distributed. We chose this distribution mostly for for computational convenience, but it is important to note that it can cover a wide range of possibilities—from a model in which every gene evolves at the same rate to a distribution so fat-tailed that there is no average rate of evolution across the group! By fitting a distribution of rates across genes in a group, we are able to look for examples of lineage-specific evolution without being confounded by outlying genes.

We encourage you to check out our paper and let us know what you think
of our approach. In addition, our method will soon be available as an
R package (once I get around to doing all the documentation…) and we
would love to see people using it. If you are interested in getting an
early version of our package, please don’t hesitate to contact me:
jgschraiber@berkeley.edu.

Our next guest post is by Mike Eisen [@mbeisen] on his paper with Peter Combs [@rflrob]
Peter A. Combs and Michael B. Eisen (2013). Sequencing mRNA from cryo-sliced Drosophila embryos to determine genome-wide spatial patterns of gene expression. arXived here.

This is cross posted from Mike’s blog.

It’s no secret to people who read this blog that I hate the way scientific publishing works today. Most of my efforts in this domain have focused on removing barriers to the access and reuse of published papers. But there are other things that are broken with the way scientists communicate with each other, and chief amongst them is pre-publication peer review. I’ve written about this before, and won’t rehash the arguments here, save to say that I think we should publish first, and then review. But one could argue that I haven’t really practiced what I preach, as all of my lab’s papers have gone through peer review before they were published.

No more. From now on we are going to post all of our papers online when we feel they’re ready to share – before they go to a journal. We’ll then solicit comments from our colleagues and use them to improve the work prior to formal publication. Physicists and mathematicians have been doing this for decades, as have an increasing number of biologists. It’s time for this to become standard practice.

Some ground rules. I will not filter comments except to remove obvious spam. You are welcome to post comments under your name or under a pseudonym – I will not reveal anyone’s identity – but I urge you to use your real name as I think we should have fully open peer review in science.

OK. Now for the paper, which is posted on arxiv and can be linked to, cited there. We also have a copy here, in case you’re having trouble with figures on arXiv.

Peter A. Combs and Michael B. Eisen (2013). Sequencing mRNA from cryo-sliced Drosophila embryos to determine genome-wide spatial patterns of gene expression.

Several years ago a postdoc in my lab, Susan Lott (now at UC Davis) developed methods to sequence the RNA’s from single Drosophila embryos. She was interested in looking at expression differences between males and females in early embryogenesis, and published a beautiful paper on that topic.

Although we were initially worried that we wouldn’t be able to get enough RNA from single embryos to get reliable sequencing results, it turns out we got more than enough. Each embryo yielded around 100ng of total RNA, and we would end up loading only ~10% of the sample onto the sequencer. So it occurred to us that maybe we could work with material from pieces of individual embryos and thereby get spatial expression information on a genomic scale in a single quick experiment – an alternative to highly informative, but slow imaging-based methods.

I recruited a new biophysics student, Peter Combs, to work on slicing embryos with a microtome along the anterior-posterior axis and sequencing each of the sections to identify genes with patterned expression along the A-P axis. In typical PI fashion, I figured this would take a few weeks, but it ended up taking over a year to get right.

The major challenge was that, while a tenth of an embyro contains more than enough RNA to analyze by mRNA-seq, it turned out to be very difficult to shepherd that RNA successfully from a single cryosection to the sequencer. Peter was routinely failing to recover RNA and make libraries from these samples using methods that worked great for whole embryos. While there are various protocols out there claiming to analyze RNA from single cells, we were reluctant to use these amplification-based strategies.

The typical way people deal with loss of small quantities of nucleic acids during experimental manipulation is to add carrier RNA or DNA – something like tRNA or salmon sperm DNA. We didn’t want to do that, since we would just end up with tons of useless sequencing reads. So we came up with a different strategy – adding embryos from distantly related Drosophila species to each slice at an early stage in the process. This brought the total amount of RNA in each sample well amove the threshold where our purification and library preparation worked robustly, and we could easily separate the D. melanogaster RNA we were interested in for this experiment from that of the “carrier” embryo. But we could avoid wasting sequencing reads by turning the carrier RNAs into an experiment of their own – in this case looking at expression variation between species.

With this trick, the method now works great, and the paper is really just a description of the method and a demonstration that accurate expression patterns can be recovered from individual cryosectioned embryos. The resolution here is not that great – we used 6 slices of ~60um each per embryo. But we’ve started to make smaller sections, and a back of the envelope calculation suggests we can, with available sample handling and sequencing techniques, make up to 100 slices per embryo. This would be more than enough to see stripes and other subtle patterns missed in the current dataset.

Our immediate near term goals are to do a developmental time course, compare patterns in male and female embryos, look at other species and examine embryos from strains carrying various patterning defects. For those of you going to the fly meeting in DC in April, Peter’s talk will, I hope, have some of this new data.

Anyway, we would love comments on either the method or the manuscript.