Project description:Myodes glareolus Raw sequence reads

Project description:Myodes glareolus Raw sequence reads

Project description:Myodes glareolus Chernobyl Transcriptome

Project description:Bank vole Myodes glareolus Genome sequencing and assembly

Project description:Myodes glareolus isolate:BV_1_Jyvaskyla Genome sequencing and assembly

Project description:Heart transcriptome of the bank vole (Myodes glareolus): towards understanding the evolutionary variation in metabolic rate

Project description:Qualitative and quantitative description of the TCRβ repertoire in bank vole (Myodes glareolus)

Project description:Study of the diversity in the repertoire size of the T-cell beta receptors in the bank vole (Myodes glareolus)

Project description:The urine of bank voles (Myodes glareolus) contains substantial quantities of a small protein that is expressed at much higher levels in males than females, and at higher levels in males in the breeding season. This protein was purified and completely sequenced at the protein level by mass spectrometry. Leucine/isoleucine ambiguity was completely resolved by metabolic labelling, monitoring the incorporation of dietary deuterated leucine into specific sites in the protein. The predicted mass of the sequenced protein was exactly consonant with the mass of the protein measured in bank vole urine samples, correcting for the formation of two disulphide bonds. The sequence of the protein revealed that it was a lipocalin related to aphrodisin and other odorant binding proteins (OBPs), but differed from all OBPs previously described. The pattern of secretion in urine used for scent marking by male bank voles, and similarity to other lipocalins used as chemical signals in rodents, suggest that this protein plays a role in male sexual and/or competitive communication. We propose the name glareosin for this novel protein to reflect the origin of the protein and to emphasise the distinction from known OBPs.

Project description:We selected normal Myodes rufocanus eyes and lens clouded eyes for transcriptome sequencing, and excavated the lens clouded eyes by analyzing and comparing. We investigated the genes and mechanisms involved in congenital cataract.