Cloning of the ACC synthase gene from Curcuma alismatifolia Gagnep. And its use in transformation studies

Cloning of the ACC synthase gene from Curcuma alismatifolia Gagnep. And its use in transformation studies

The goal of this work was to suppress the expression of the ACC synthase gene in the Siam tulip, Curcuma alismatifolia Gagnep. A cDNA fragment encoding ACC synthase from C. alismatifolia Gagnep. was isolated and expression studies were done. To isolate this gene a pair of primers was designed from t...

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Main Authors: S. Mahadtanapuk, M. Sanguansermsri, T. Handa, W. Nanakorn, S. Anuntalabhochai
Format: Book Series
Published: 2018
Subjects:
Agricultural and Biological Sciences
Online Access:https://www.scopus.com/inward/record.uri?partnerID=HzOxMe3b&scp=75649100067&origin=inward
http://cmuir.cmu.ac.th/jspui/handle/6653943832/48821
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Institution: Chiang Mai University
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spelling th-cmuir.6653943832-488212018-08-16T01:57:46Z Cloning of the ACC synthase gene from Curcuma alismatifolia Gagnep. And its use in transformation studies S. Mahadtanapuk M. Sanguansermsri T. Handa W. Nanakorn S. Anuntalabhochai Agricultural and Biological Sciences The goal of this work was to suppress the expression of the ACC synthase gene in the Siam tulip, Curcuma alismatifolia Gagnep. A cDNA fragment encoding ACC synthase from C. alismatifolia Gagnep. was isolated and expression studies were done. To isolate this gene a pair of primers was designed from the highly conserved motif of ACC synthases in various plant species. The PCR product of 600 bp. in C. alismatifolia Gagnep. was subcloned into the pGEM-T easy vector resulting in pCa-ACSI. After sequencing, the sequence and its deduced amino acid sequence were highly homologous to the ACC synthases from other plants. To determine expression patterns of pCa-ACSI, a Northern blot analysis showed that the expression of the pCa-ACSI gene was in the bracts of curcuma, the highest expression was observed 2 days after cutting the flowers. Ca-ACSI was subcloned in pBI121 resulting in pBI121-Ca-ACSI and transformed into leaf tissues of Torenia foumieri and retarded shoots of C. alismatifolia Gagnep via Agrobacterium tumefaciens strain AGLO. Putative transformants, with the gene in an antisense orientation, were investigated by PCR analysis, GUS assays and Southern blotting. The transgenic plantlets were transferred to pots containing soil for cultivation in growth chamber. At present, the transgenic plants grow happily in the greenhouse and their phenotypic is under investigation. 2018-08-16T01:57:46Z 2018-08-16T01:57:46Z 2009-01-01 Book Series 05677572 2-s2.0-75649100067 10.17660/ActaHortic.2009.836.40 https://www.scopus.com/inward/record.uri?partnerID=HzOxMe3b&scp=75649100067&origin=inward http://cmuir.cmu.ac.th/jspui/handle/6653943832/48821
institution Chiang Mai University
building Chiang Mai University Library
country Thailand
collection CMU Intellectual Repository
topic Agricultural and Biological Sciences
spellingShingle Agricultural and Biological Sciences
S. Mahadtanapuk
M. Sanguansermsri
T. Handa
W. Nanakorn
S. Anuntalabhochai
Cloning of the ACC synthase gene from Curcuma alismatifolia Gagnep. And its use in transformation studies
description The goal of this work was to suppress the expression of the ACC synthase gene in the Siam tulip, Curcuma alismatifolia Gagnep. A cDNA fragment encoding ACC synthase from C. alismatifolia Gagnep. was isolated and expression studies were done. To isolate this gene a pair of primers was designed from the highly conserved motif of ACC synthases in various plant species. The PCR product of 600 bp. in C. alismatifolia Gagnep. was subcloned into the pGEM-T easy vector resulting in pCa-ACSI. After sequencing, the sequence and its deduced amino acid sequence were highly homologous to the ACC synthases from other plants. To determine expression patterns of pCa-ACSI, a Northern blot analysis showed that the expression of the pCa-ACSI gene was in the bracts of curcuma, the highest expression was observed 2 days after cutting the flowers. Ca-ACSI was subcloned in pBI121 resulting in pBI121-Ca-ACSI and transformed into leaf tissues of Torenia foumieri and retarded shoots of C. alismatifolia Gagnep via Agrobacterium tumefaciens strain AGLO. Putative transformants, with the gene in an antisense orientation, were investigated by PCR analysis, GUS assays and Southern blotting. The transgenic plantlets were transferred to pots containing soil for cultivation in growth chamber. At present, the transgenic plants grow happily in the greenhouse and their phenotypic is under investigation.
format Book Series
author S. Mahadtanapuk
M. Sanguansermsri
T. Handa
W. Nanakorn
S. Anuntalabhochai
author_facet S. Mahadtanapuk
M. Sanguansermsri
T. Handa
W. Nanakorn
S. Anuntalabhochai
author_sort S. Mahadtanapuk
title Cloning of the ACC synthase gene from Curcuma alismatifolia Gagnep. And its use in transformation studies
title_short Cloning of the ACC synthase gene from Curcuma alismatifolia Gagnep. And its use in transformation studies
title_full Cloning of the ACC synthase gene from Curcuma alismatifolia Gagnep. And its use in transformation studies
title_fullStr Cloning of the ACC synthase gene from Curcuma alismatifolia Gagnep. And its use in transformation studies
title_full_unstemmed Cloning of the ACC synthase gene from Curcuma alismatifolia Gagnep. And its use in transformation studies
title_sort cloning of the acc synthase gene from curcuma alismatifolia gagnep. and its use in transformation studies
publishDate 2018
url https://www.scopus.com/inward/record.uri?partnerID=HzOxMe3b&scp=75649100067&origin=inward
http://cmuir.cmu.ac.th/jspui/handle/6653943832/48821
_version_ 1681423299075112960

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