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Mutation of a Cuticle Protein Gene, BmCPG10, Is Responsible for Silkworm Non-Moulting in the 2(nd) Instar Mutant

In the silkworm, metamorphosis and moulting are regulated by ecdysone hormone and juvenile hormone. The subject in the present study is a silkworm mutant that does not moult in the 2(nd) instar (nm2). Genetic analysis indicated that the nm2 mutation is controlled by a recessive gene and is homozygou...

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Autores principales: Wu, Fan, Wang, Pingyang, Zhao, Qiaoling, Kang, Lequn, Xia, Dingguo, Qiu, Zhiyong, Tang, Shunming, Li, Muwang, Shen, Xingjia, Zhang, Guozheng
Formato: Online Artículo Texto
Lenguaje:English
Publicado: Public Library of Science 2016
Materias:
Acceso en línea:https://www.ncbi.nlm.nih.gov/pmc/articles/PMC4838254/
https://www.ncbi.nlm.nih.gov/pubmed/27096617
http://dx.doi.org/10.1371/journal.pone.0153549
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author Wu, Fan
Wang, Pingyang
Zhao, Qiaoling
Kang, Lequn
Xia, Dingguo
Qiu, Zhiyong
Tang, Shunming
Li, Muwang
Shen, Xingjia
Zhang, Guozheng
author_facet Wu, Fan
Wang, Pingyang
Zhao, Qiaoling
Kang, Lequn
Xia, Dingguo
Qiu, Zhiyong
Tang, Shunming
Li, Muwang
Shen, Xingjia
Zhang, Guozheng
author_sort Wu, Fan
collection PubMed
description In the silkworm, metamorphosis and moulting are regulated by ecdysone hormone and juvenile hormone. The subject in the present study is a silkworm mutant that does not moult in the 2(nd) instar (nm2). Genetic analysis indicated that the nm2 mutation is controlled by a recessive gene and is homozygous lethal. Based on positional cloning, nm2 was located in a region approximately 275 kb on the 5(th) linkage group by eleven SSR polymorphism markers. In this specific range, according to the transcriptional expression of thirteen genes and cloning, the relative expression level of the BmCPG10 gene that encodes a cuticle protein was lower than the expression level of the wild-type gene. Moreover, this gene’s structure differs from that of the wild-type gene: there is a deletion of 217 bp in its open reading frame, which resulted in a change in the protein it encoded. The BmCPG10 mRNA was detectable throughout silkworm development from the egg to the moth. This mRNA was low in the pre-moulting and moulting stages of each instar but was high in the gluttonous stage and in newly exuviated larvae. The BmCPG10 mRNA showed high expression levels in the epidermis, head and trachea, while the expression levels were low in the midgut, Malpighian tubule, prothoracic gland, haemolymph and ventral nerve cord. The ecdysone titre was determined by ELISA, and the results demonstrated that the ecdysone titre of nm2 larvae was lower than that of the wild-type larvae. The nm2 mutant could be rescued by feeding 20-hydroxyecdysone, cholesterol and 7—dehydrocholesterol (7dC), but the rescued nm2 only developed to the 4(th) instar and subsequently died. The moulting time of silkworms could be delayed by BmCPG10 RNAi. Thus, we speculated that the mutation of BmCPG10 was responsible for the silkworm mutant that did not moult in the 2(nd) instar.
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spelling pubmed-48382542016-04-29 Mutation of a Cuticle Protein Gene, BmCPG10, Is Responsible for Silkworm Non-Moulting in the 2(nd) Instar Mutant Wu, Fan Wang, Pingyang Zhao, Qiaoling Kang, Lequn Xia, Dingguo Qiu, Zhiyong Tang, Shunming Li, Muwang Shen, Xingjia Zhang, Guozheng PLoS One Research Article In the silkworm, metamorphosis and moulting are regulated by ecdysone hormone and juvenile hormone. The subject in the present study is a silkworm mutant that does not moult in the 2(nd) instar (nm2). Genetic analysis indicated that the nm2 mutation is controlled by a recessive gene and is homozygous lethal. Based on positional cloning, nm2 was located in a region approximately 275 kb on the 5(th) linkage group by eleven SSR polymorphism markers. In this specific range, according to the transcriptional expression of thirteen genes and cloning, the relative expression level of the BmCPG10 gene that encodes a cuticle protein was lower than the expression level of the wild-type gene. Moreover, this gene’s structure differs from that of the wild-type gene: there is a deletion of 217 bp in its open reading frame, which resulted in a change in the protein it encoded. The BmCPG10 mRNA was detectable throughout silkworm development from the egg to the moth. This mRNA was low in the pre-moulting and moulting stages of each instar but was high in the gluttonous stage and in newly exuviated larvae. The BmCPG10 mRNA showed high expression levels in the epidermis, head and trachea, while the expression levels were low in the midgut, Malpighian tubule, prothoracic gland, haemolymph and ventral nerve cord. The ecdysone titre was determined by ELISA, and the results demonstrated that the ecdysone titre of nm2 larvae was lower than that of the wild-type larvae. The nm2 mutant could be rescued by feeding 20-hydroxyecdysone, cholesterol and 7—dehydrocholesterol (7dC), but the rescued nm2 only developed to the 4(th) instar and subsequently died. The moulting time of silkworms could be delayed by BmCPG10 RNAi. Thus, we speculated that the mutation of BmCPG10 was responsible for the silkworm mutant that did not moult in the 2(nd) instar. Public Library of Science 2016-04-20 /pmc/articles/PMC4838254/ /pubmed/27096617 http://dx.doi.org/10.1371/journal.pone.0153549 Text en © 2016 Wu et al http://creativecommons.org/licenses/by/4.0/ This is an open access article distributed under the terms of the Creative Commons Attribution License (http://creativecommons.org/licenses/by/4.0/) , which permits unrestricted use, distribution, and reproduction in any medium, provided the original author and source are credited.
spellingShingle Research Article
Wu, Fan
Wang, Pingyang
Zhao, Qiaoling
Kang, Lequn
Xia, Dingguo
Qiu, Zhiyong
Tang, Shunming
Li, Muwang
Shen, Xingjia
Zhang, Guozheng
Mutation of a Cuticle Protein Gene, BmCPG10, Is Responsible for Silkworm Non-Moulting in the 2(nd) Instar Mutant
title Mutation of a Cuticle Protein Gene, BmCPG10, Is Responsible for Silkworm Non-Moulting in the 2(nd) Instar Mutant
title_full Mutation of a Cuticle Protein Gene, BmCPG10, Is Responsible for Silkworm Non-Moulting in the 2(nd) Instar Mutant
title_fullStr Mutation of a Cuticle Protein Gene, BmCPG10, Is Responsible for Silkworm Non-Moulting in the 2(nd) Instar Mutant
title_full_unstemmed Mutation of a Cuticle Protein Gene, BmCPG10, Is Responsible for Silkworm Non-Moulting in the 2(nd) Instar Mutant
title_short Mutation of a Cuticle Protein Gene, BmCPG10, Is Responsible for Silkworm Non-Moulting in the 2(nd) Instar Mutant
title_sort mutation of a cuticle protein gene, bmcpg10, is responsible for silkworm non-moulting in the 2(nd) instar mutant
topic Research Article
url https://www.ncbi.nlm.nih.gov/pmc/articles/PMC4838254/
https://www.ncbi.nlm.nih.gov/pubmed/27096617
http://dx.doi.org/10.1371/journal.pone.0153549
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