Hi,

I was wondering if there is a way to decide what kind of p-value will be the right one to identify differentially expressed genes.

I am running a microarray analysis and using the LIMMA package for the identification of those DEG. I am getting a table with the toptable command. I have a table of almost 10000 genes.

How do I know where to set the parameter for a p-valueas a threshold?

I read quite a few papers about it and there is basically no consensus. Most of the people set p<0.01 as one, but by doing so I don't get much of data. IS there a way of analyzing/plotting the p-values to get a better overview of the "right" p-value?

Assuming that you are using the defaults and that you are talking about using the adj.p.val, there is a natural and intuitive interpretation. The adjusted p-value is actually a false discovery rate. The natural interpretation is that at 0.01, one out of 100 genes in the list are likely to be false discoveries. At 0.05, five out of 100 in the list are likely false discoveries. What is the best cutoff? It depends. But using the concept of the false discovery rate, you can see that a given cutoff leads to a natural interpretation of the results.

As for your particular experiment, 10000 genes that show differential expression at adj.p.value of 0.01 seems pretty high, but it might make sense for your experiment. Have you looked at a heatmap of your results? Do they make sense?

There is no consensus because there is no "right" p-value. Remember that the p-values you are calculating are based on assumptions. Assumptions that the distribution of the data has a certain shape, that the variability of your replicates has a certain distribution. The p-value represents a fractional area from the shape of a distribution - which may or may not fit your data very well. Experiments of this kind have many variables (that you may be unaware of) such that microarrays can give data distributions that are significantly different from what one might expect. I've seen experiments that return no "good" p-values, that a statistician declares a failed experiment, yet as a biologist I can see a gold mine of information there. In these cases, realize that your treatment is based on assumptions (that you probably haven't or don't know how to test), and simply use the p-values as a ranking mechanism - and forget about absolute magnitude. Be a good experimentalist and look for any signal in the data which makes biological sense (as other have suggested, use gene set analysis, or find any predictable marker gene), so you can decide if there is anything there, and perhaps how you can do a better experiment next time. On the other hand, if there is nothing there, it may be a truly worthless experiment and you'll waste time trying to mine bad data, chasing false leads. P-values are not magic, they are areas under a curve that may or may not be relevant to your data. Follow Sean's and Davy's and Neal's suggestions, explore the shapes, be a good experimentalist, be a skeptical biologist.

To get an idea of the distribution of your p-values you could use:

tT <- topTable(fit2, adjust.method="fdr", number=nfow(fit2))

Then plot

x <- -log10(tT$adj.p.val)
plot(x, type="l")
sigline <- c(.05, .01, .005, .001,.0005, .0001)
sigline <- -log10(sigline)
sigcolors <- c("red", "blue", "green", "yellow","pink","purple")
sapply(1:length(sigline), function(x){abline(h=sigline[x], col=sigcolors[x])})

Not getting a large list of genes that are differentially expressed might actually be a good thing depending on what genes they are and the conditions you are comparing. See the following blog for an idea about what you can do with your data afterwards:

http://gettinggeneticsdone.blogspot.com/2012/03/pathway-analysis-for-high-throughput.html

we're comparing mouse microarrays of knock-out mice vs. wild-type. I have three replicates for each treatment. (I know this is not much, but this is what we've got. we are interested in prolonged life expansion due to several KO-mutants.

Some of the genes we are interested in shows a "good" behavior. With that I mean for example, that they show differential expression in the way we expected them to have. The problem is, that the significance depends on the threshold I am going to choose. The genes we are looking for have partially a adj.P.Val higher than the threshold of 0.05, but lower than 0.1. So If I choose the 0.05 the genes will be unimportant, but with 0.1 they will be o.k.

The problem is not what the right one, as I already understood there is no right one, but more important is how to explain the decision to take the 0.1 threshold, besides just saying it fits better to the experiment.

Is there a statistical/methodical way of explaining the threshold chosen?

Thanks

PS I uploaded the image of the example Sean provided. cut-off graph

Hi Sean, Frymor and Davy,

I am a newbie to microarray data analysis. I've got a data set of microarrays to work on. I was able to run the rma normalization and LIMMA analysis.

Now I have a big table of over 25K genes. If I understood it correctly most of them are not differentially regulated. The question is of course, how to identify the genes which are significant?

I was using the example offered here to plot my data and got the same curve and lines of p-values. Am I wrong to understand that this plot is the same as the histogram of the p-values distribution which is easily done by various examples and shows a something like this: histogram - image was taken from http://www.tcrt.org But, now that I have it, what do I do with it?

I know that the plot shows me the distribution of the p-values over my experiments. The person I am working with told me I need to look for the point, where the curve goes flat-lined, but this is as arbitrary as just picking a p-value by chance. His reason for that choice was - everybody is doing so. This is what I understood after reading some papers -

1. In a normal experiment most of the genes won't be differentially regulated.
2. the adj. p-value is my multiple testing hypothesis correction value.
3. the higher this value is, the more false positive I get in my list of DE genes.

But all these doesn't help me to find the right threshold. I read this paper: Estimating p-values in small microarray experiments. Here they try to explain why permutations is a good idea with small data sets (which I also have - four replicates for three different conditions each). But still not a clue about the 'right' value

> You are not going to get an answer from this group on the question of what the right number is because there is no one-size-fits-all number to use. If you are unclear about how to interpret your results, I suggest you find a local collaborator who can work with you on your data.

I can understand Sean's saying it is difficult to get an answer to such a question, as there is no straight or direct answer for that. Each experiment is a single, unique data set. But I am sure there is some kind of method to define the right p-value by looking at the distribution of the data. AN explanation might be that I am to choose the point where the curve is getting flatter for the reason that at this point I will have the highest number of significantly differentially regulated genes with the smaller number of false positive in this data.

Is this an explanation which can stand?

Thanks for the help?

Alex