Is there an easy, inexpensive, not too labor intensive way to normalise mRNA samples so that even though one loses information of gene expression levels, each of the transcripts in the transcriptome is equally represented in the sample for sequencing? This is to say, one has a uniform distribution of transcripts, so that the lowly-expressed transcripts still have a good chance of being sequenced.

I have seen a few papers mentioning protocols for mRNA normalization, but I can't tell if any of them is practical in real life wet lab situations.

There is some talk of normalization by use of a duplex specific nuclease (DSN). This has been discussed in several threads on SeqAnswers here. Another option is to take your cDNA library, capture it with a capture reagent (e.g. exome array or liquid capture kit), and then sequence it. This will reduce the representation of highly expressed transcripts in your library and allow your library depth to be spread more evenly across the transcriptome.

Have you looked at Springer protocols: Accessing the transcriptome: how to normalize mRNA pools ?

http://www.ncbi.nlm.nih.gov/pubmed/22065434

Thanks @Malachig for your DSN link. I found the link to the commercial product by Evrogen here:
http://www.evrogen.com/technologies/normalization.shtml

They claim their method is compatible with nextgen sequencing platforms:

cDNA normalization using duplex-specific nuclease (DSN) is a highly efficient approach that can be applied for normalization of full-length-enriched cDNA (Zhulidov et al., 2004; Zhulidov et al., 2005). The resulting cDNA contains equalized abundance of different transcripts and can be used for construction of cDNA libraries and for direct sequencing, including high-throughput sequencing on the next generation sequencing platforms (Roche/454, ABI/SOLiD or Illumina/Solexa).

And the most up-to-date reference seems to be this Curr Protoc Mol Biol. paper by Bogdanova et al.:
http://www.ncbi.nlm.nih.gov/pubmed/20373503