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  4. Effects of rho-independent terminators on the expression of the prokaryotic β-glucuronidase gene in tobacco
 
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Effects of rho-independent terminators on the expression of the prokaryotic β-glucuronidase gene in tobacco

Resource
Physiologia Plantarum 108 (2): 171-179
Journal
Physiologia Plantarum
Journal Volume
108
Journal Issue
2
Pages
171-179
Date Issued
2000
Date
2000
Author(s)
Jeng, Shih-Tong  
Yen, Chia-Yu
DOI
10.1034/j.1399-3054.2000.108002171.x
URI
http://ntur.lib.ntu.edu.tw//handle/246246/162055
https://www.scopus.com/inward/record.uri?eid=2-s2.0-0034010925&doi=10.1034%2fj.1399-3054.2000.108002171.x&partnerID=40&md5=5c66679dba9ae373e9b2b1dacc8f34e0
Abstract
The threonine (thr) attenuator with a dyad symmetrical structure is from the regulatory region of the thr operon of Escherichia coli, and encodes RNA with a stem-and-loop structure followed by a stretch of uridine residues. The thr attenuator and its variants were subcloned into the region between the 35S promoter and β-glucuronidase (GUS) coding region, and the transient expression of GUS gene in tobacco protoplast was treated as a reporter for gene regulation in plants. Results from the 14 variants in the stem region of the thr attenuator indicated that both base pairing and sequence specificity in the G + C-rich region of the stem were important for the GUS expression, but 1 base mismatch in the A + U-rich region of stem did not affect the GUS expression in plants. Seven variants with nested deletion in the stretch of uridine residues were also analyzed, and the results suggested that the variants with the shorter uridine stretch produced more GUS protein than those with the longer stretch. Transgenic tobacco plants with the thr attenuator and its variants located between the 35S promoter and GUS coding region were also generated, and their steady state RNAs were hybridized with 2 radioactive antisense RNA probes which bound 5' and 3' of the thr hairpin, respectively. After the digestion of S1 nuclease, the amount of the nuclease-resistant transcript from the protection of the 5' antisense RNA probe was much more than that from the protection of the 3' probe in all tested variants. This result suggests that these dyad symmetries may affect transcription of plant RNA polymerase II.
Other Subjects
antisense RNA; base pairing; gene deletion; genetic variance; operon; promoter region; protoplast; regulator gene; reporter gene; tobacco; transcription termination; transgenic plant; Escherichia coli
Type
journal article
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