---
author: einar
categories:
- Science
comments: true
date: "2008-02-28T19:42:15Z"
header:
  image_fullwidth: banner_other.jpg
slug: follow-up-on-meta-analysis
tags:
- meta-analysis
- microarray
- Science
title: Follow up on meta-analysis
omit_header_text: true
disable_share: true
wordpress_id: 378
---

Fourteen days since my last post. Quite a while, indeed. Mostly I've been stumbled with work and some health related issues. Anyway, I thought I'd follow up on the meta analysis matter I discussed in my last post.

It turns out that it's a fault of both limma and the data sets, because apparently the raw data found in the Stanford Microarray Database have different length, gene-wise (a result of not all spots on the array being good?) and limma itself does need equal length tables to form a single object (I stumbled upon the same problem when doing my thesis, but I used a hack to work around it), and does not perform any checking.

According to the documentation, the "merge" command should be used to deal with these cases, but here's what I get:

{{< highlight R >}}

>> RG1 = read.maimages(file="file1.txt",source="smd")
Read file1.txt
>> RG2 = read.maimages(file="file2.txt",source="smd")
Read file2.txt
>> merge(RG1,RG2)
Error in merge(RG1,RG2): Need row names to align on
>> rownames(RG1)
NULL
>> rownames(RG2)
NULL 
{{< / highlight >}}

I'm going to ask the Bioconductor ML and see what they tell me.