Multiple functions of precursor BDNF to CNS neurons: negative regulation of neurite growth, spine formation and cell survival

Hisatsugu Koshimizu; Kazuyuki Kiyosue; Tomoko Hara; Shunsuke Hazama; Shingo Suzuki; Koichi Uegaki; Guhan Nagappan; Eugene Zaitsev; Takatsugu Hirokawa; Yoshiro Tatsu; Akihiko Ogura; Bai Lu; Masami Kojima

doi:10.1186/1756-6606-2-27

Multiple functions of precursor BDNF to CNS neurons: negative regulation of neurite growth, spine formation and cell survival

Hisatsugu Koshimizu(National Institute of Advanced Industrial Science and Technology), Kazuyuki Kiyosue(National Institute of Advanced Industrial Science and Technology), Tomoko Hara(Japan Science and Technology Agency), Shunsuke Hazama(National Institute of Advanced Industrial Science and Technology), Shingo Suzuki(Japan Science and Technology Agency), Koichi Uegaki(Japan Science and Technology Agency), Guhan Nagappan(National Institutes of Health), Eugene Zaitsev(National Institutes of Health), Takatsugu Hirokawa(Japan Science and Technology Agency), Yoshiro Tatsu(Japan Science and Technology Agency), Akihiko Ogura(The University of Osaka), Bai Lu(National Institutes of Health), Masami Kojima(Japan Science and Technology Agency)

Molecular Brain

August 13, 2009

10.1186/1756-6606-2-27

Cited by 195Open Access

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Abstract

BACKGROUND: Proneurotrophins and mature neurotrophins elicit opposite effects via the p75 neurotrophin receptor (p75(NTR)) and Trk tyrosine kinase receptors, respectively; however the molecular roles of proneurotrophins in the CNS are not fully understood. RESULTS: Based on two rare single nucleotide polymorphisms (SNPs) of the human brain-derived neurotrophic factor (BDNF) gene, we generated R125M-, R127L- and R125M/R127L-BDNF, which have amino acid substitution(s) near the cleavage site between the pro- and mature-domain of BDNF. Western blot analyses demonstrated that these BDNF variants are poorly cleaved and result in the predominant secretion of proBDNF. Using these cleavage-resistant proBDNF (CR-proBDNF) variants, the molecular and cellular roles of proBDNF on the CNS neurons were examined. First, CR-proBDNF showed normal intracellular distribution and secretion in cultured hippocampal neurons, suggesting that inhibition of proBDNF cleavage does not affect intracellular transportation and secretion of BDNF. Second, we purified recombinant CR-proBDNF and tested its biological effects using cultured CNS neurons. Treatment with CR-proBDNF elicited apoptosis of cultured cerebellar granule neurons (CGNs), while treatment with mature BDNF (matBDNF) promoted cell survival. Third, we examined the effects of CR-proBDNF on neuronal morphology using more than 2-week cultures of basal forebrain cholinergic neurons (BFCNs) and hippocampal neurons. Interestingly, in marked contrast to the action of matBDNF, which increased the number of cholinergic fibers and hippocampal dendritic spines, CR-proBDNF dramatically reduced the number of cholinergic fibers and hippocampal dendritic spines, without affecting the survival of these neurons. CONCLUSION: These results suggest that proBDNF has distinct functions in different populations of CNS neurons and might be responsible for specific physiological cellular processes in the brain.

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