Correct splicing of a group II intron from a chimeric reporter gene transcript in tobacco plastids

doi:10.1093/nar/23.13.2544

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Nucleic Acids Research, 1995, Vol. 23, No. 13 2544-2547
© 1995

METHODS

Correct splicing of a group II intron from a chimeric reporter gene transcript in tobacco plastids

Ralph Bock⁺ and Pal Maliga^*

Waksman Institute, Rutgers, The State University of New Jersey PO Box 759, Old Hoes Lane, Piscataway, NJ 08855–0759, USA

^*To whom correspondence should be addressed

Received February 8, 1995. Accepted May 10, 1995.

A in vivo test system was developed to study group II Intronsplicing in higher plant chloroplasts. The chimeric reportergene uldA^* was constructed by translatlonal fusion of an intron-containlngsegment of the plastld atpF gene with the coding region of aplastld uldA reporter gene. The chimeric uldA^* gene was insertedinto the tobacco plastid genome by the biollstlc transformationprocedure using a plastid targeting vector. Correct intron excisionwas confirmed by Northern blot analysis, by sequencing amplifiedDNAs and by accumulation of the encoded fi-glucuronldase (GUS),the expression of which was dependent on intron removal. Removalof the intron from the uldA^*mRNA is less efficient (<50%)than from the atpF mRNA (>90%). The efficiency of atpF mRNAsplicing is not affected in the plastid transformants Indicatingthat inefficient splicing of the highlyexpressed uldA^* mRNAis not due to depletion of factors) required for the atpF intronremoval. A derivative of uldA^*, with a stop codon introducedinto the loop of domain VI, was also tested. The mutations didnot affect the splicing efficiency. The chimeric uldA^* splicingsystem will facilitate the study of structural and sequencerequirements for group II Intron splicing in plastids of higherplants.

⁺Present address: Institut für Biologie III, UniversitätFreiburg, Schänzlestraße 1, D-79104 Freiburg,Germany

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