1984
DOI: 10.1016/0092-8674(84)90432-x
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The use of promoter fusions in Drosophila genetics: Isolation of mutations affecting the heat shock response

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Cited by 177 publications
(74 citation statements)
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“…The reporter construct, herein called pOCA108, contains two full-length CAB3 promoters (see details in Susek et al, 1993) fused to either the alcohol dehydrogenase (ADH) gene from Arabidopsis (Chang and Meyerowitz, 1986) or the Escherichia coli 0-glucuronidase (&A, or GUS) gene (Jefferson, 1987). We chose ADH because both positive and negative genetic selections exist for this enzyme (Bonner et al, 1984). This was important to our screen because we could select against ADH activity using allyl alcohol, which is converted into the toxic aldehyde acrolein.…”
Section: Mutant Lsolation and Genetic Characterizationmentioning
confidence: 99%
“…The reporter construct, herein called pOCA108, contains two full-length CAB3 promoters (see details in Susek et al, 1993) fused to either the alcohol dehydrogenase (ADH) gene from Arabidopsis (Chang and Meyerowitz, 1986) or the Escherichia coli 0-glucuronidase (&A, or GUS) gene (Jefferson, 1987). We chose ADH because both positive and negative genetic selections exist for this enzyme (Bonner et al, 1984). This was important to our screen because we could select against ADH activity using allyl alcohol, which is converted into the toxic aldehyde acrolein.…”
Section: Mutant Lsolation and Genetic Characterizationmentioning
confidence: 99%
“…pCR2 has a XbaI-HmdIII fragment containing the alcohol dehydrogenase structural gene from D. melanogaster (Bonner et al 1984) fused at its HindIII site in the nontranslated leader region to the AvaII site in ypl (+37 of ypl) through a linker (5'-AAGAGGGCTGCAAAGCTCTCTAGAGGTCCTGCGG-3'; the fusion site was verified by sequencing; underlining indicates the Adh sequence beginning at + 21 relative to the larval cap site and the modified HindIII and AvaII sites in 5' to 3' order). The yolk protein component of pCR2 extends to the NcoI site in yp2 ( + 105 of yp2), which is fused to the Sinai site of a modified E. coli lacZ gene [pMLB1034(&AvaI) ~ Shapira et al 1983] by a linker (5'-GCCATGCGGTCGACCGGGGATCCC-3'; underlining indicates the NcoI and SmaI sites remaining in pCR2).…”
Section: Construction Of P-element Plasmidsmentioning
confidence: 99%
“…First, the 5Ј-untranslated region (5Ј-UTR) of Hsp mRNAs is sufficient to confer efficient translation to a heterologous appended coding region (10,11); and conversely, the Hsp coding sequence and 3Ј-UTR are unable to be translated during heat shock when a non-heat shock 5Ј-UTR, or a mutationally disabled Hsp 5Ј-UTR, precedes it (12,13). Second, the common features found in virtually all Drosophila Hsp mRNA 5Ј-UTRs include: (i) long length (200 -250 nucleotides); (ii) two conserved sequence segments, and positionally conserved nucleotides within the initial element; (iii) a high frequency of adenosine nucleotides (ϳ50%); and (iv) a minimal extent of secondary structure (7).…”
mentioning
confidence: 99%