Proteomics and signal transduction in the crustacean molting gland

doi:10.1093/icb/icl047

Integrative and Comparative Biology Advance Access published online on October 3, 2006
Integrative and Comparative Biology, doi:10.1093/icb/icl047

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© The Author 2006. Published by Oxford University Press on behalf of the Society for Integrative and Comparative Biology. All rights reserved. For permissions please email: journals.permissions@oxfordjournals.org.

Genomic and Proteomic Approaches in Crustacean Biology

Proteomics and signal transduction in the crustacean molting gland

Sung Gu Lee ¹ and Donald L. Mykles ¹ ^*
¹ Department of Biology, Colorado State University, Fort Collins, CO 80523, USA

^* To whom correspondence should be addressed.
Donald L. Mykles, E-mail: don{at}lamar.colostate.edu

Abstract

Synopsis Regulation of the molting cycle in decapod crustaceansinvolves 2 endocrine organs: the X-organ/sinus gland (XO/SG)complex located in the eyestalk ganglia and the Y-organ (YO)located in the cephalothorax. Two neuropeptides [molt-inhibitinghormone (MIH) and crustacean hyperglycemic hormone (CHH)] areproduced in the XO/SG complex and inhibit ecdysteroidogenesisin the YO. Thus, YO activation is induced by eyestalk ablation(ESA), which removes the primary source of MIH and CHH. Cyclicnucleotides (cAMP and cGMP) and nitric oxide (NO) appear tomediate neuropeptide suppression of the YO. Proteomics was usedto identify potential components of signal transduction pathways("targeted" or cell-map proteomics) as well as assess the magnitudeof protein changes in response to activation ("global" or expressionproteomics) in the tropical land crab, Gecarcinus lateralis.Total proteins in YOs from intact and ES-ablated animals wereseparated by two-dimensional gel electrophoresis and expressionprofiles were assessed by image analysis and gene clusteringsoftware. ESA caused a >3-fold increase in the levels of170 proteins and >3-fold decrease in the levels of 89 proteins;a total of 543 proteins were quantified in total YO extracts.ESA induced significant changes in the levels of 3 groups ofproteins eluting from a phosphoprotein column and detected withphosphoprotein staining of two-dimensional gels; $~$ 17 kDa and $~$ 150 kDa phosphoproteins increased in activated YOs, while $~$ 12kDa phosphoproteins decreased. A $~$ 150 kDa phosphoprotein, whichwas isolated only from activated YO, was identified as NO synthaseby western blotting and mass spectrometry of trypsin peptides.These data show that phosphorylation of NO synthase is associatedwith activation of the YO. A neuropeptide signaling pathwayinvolving NO synthase and NO-sensitive guanylyl cyclase is proposed.

From the symposium "Genomic and Proteomic Approaches in Crustacean Biology" presented at the annual meeting of the Society for Integrative and Comparative Biology, January 4-8, 2006, at Orlando, Florida.

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This article has been cited by other articles:

S. G. Lee, B. D. Bader, E. S. Chang, and D. L. Mykles
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