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- Bookedited by Christopher Peacock, University of Western Australia, Nedlands, WA, Australia.Contents:
The eukaryotic pathogen databases : a functional genomic resource integrating data from human and veterinary parasites
From sequence mapping to genome assemblies
Sequencing and annotation of mitochondrial genomes from individual parasitic helminths
A beginners guide to estimating the non-synonymous to synonymous rate ratio of all protein-coding genes in a genome
Exploiting genetic variation to discover genes involved in important disease phenotypes
Identification and analysis of ingi-related retroposons in the trypanosomatid genomes
Approaches for studying mRNA decay mediated by SIDER2 retroposons in Leishmania
Gene suppression in schistosomes using RNAi
Construction of Trypanosoma brucei illumina RNA-seq libraries enriched for transcript ends
Techniques to study epigenetic control and the epigenome in parasites
The genome-wide identification of promotor regions in Toxoplasma gondii
RNA-seq approaches for determining mRNA abundance in Leishmania
Protein microarrays for parasite antigen discovery
A transposon-based tool for transformation and mutagenesis in Trypanosomatid protozoa
Separation of basic proteins from Leishmania using a combination of free flow electrophoresis (FFE) and 2D electrophoresis (2-DE) under basic conditions
Proteomic analysis of posttranslational modifications using iTRAQ in Leishmania
Large-scale differential proteome analysis in Plamsmodium falciparum under drug treatment
Use of ¹³C stable isotope labelling for pathway and metabolic flux analysis in Leishmania parasites
Molecular genotyping of Trypanosoma cruzi for lineage assignment and population genetics
Screening Leishmania donovani complex-specific genes required for visceral disease.Digital Access Springer 2015 - ArticleElimination of cobalt from the frog brain introduced into the optic centres through the optic nerve.Lázár G.Acta Biol Acad Sci Hung. 1979;30(3):245-55.One optic nerve in several frogs was filled with cobaltous-lysine complex, and the animals were left to survive from 1 day to 52 days. Degenerated cobalt-filled retinal fibres were phagocytosed by ependymo-glial, and microglial cells. The cobalt appeared in the ependymo-glial cells in the 4th postoperative day, and its amount was greatly reduced by the 52nd day. Within 12 days the labelled axons were replaced by cobalt-loaded microglial cells in the termination sites of optic fibres. By the end of the experimental period, the number of labelled cells increased in the periventricular layers, and decreased in places where retinal fibres had terminated. These processes were accompanied by the appearance of cobalt in the choroid plexus. It is supposed that glial cells dischargd the cobalt into brain ventricles, and the metal left the nervous tissue via the cerebrospinal fluid.