Fig. 6.
Fig. 6. Sequence analysis of p67-phox cDNA in patients SG and CG. The region between exons 10 and 14 was amplified by PCR using primers p67-835LcDNA and p67-1102RcDNA. The upper panel of the figure shows the cDNA sequences of a normal control and patients SG and CG with the 3′ end at the top. The dashed line indicates the 3′ end of exon 10 and the beginning of 2 different sequences in each patient. The lower panel of the figure shows a schematic representation of the splice defect produced by the nt substitution in the branch point sequence of intron 10. The A → G transition at position −21 of intron 10, important for RNA lariat formation, produces a partial defect in splicing of exon 11 that can allow alternative splicing between exons 10 and 12.

Sequence analysis of p67-phox cDNA in patients SG and CG. The region between exons 10 and 14 was amplified by PCR using primers p67-835LcDNA and p67-1102RcDNA. The upper panel of the figure shows the cDNA sequences of a normal control and patients SG and CG with the 3′ end at the top. The dashed line indicates the 3′ end of exon 10 and the beginning of 2 different sequences in each patient. The lower panel of the figure shows a schematic representation of the splice defect produced by the nt substitution in the branch point sequence of intron 10. The A → G transition at position −21 of intron 10, important for RNA lariat formation, produces a partial defect in splicing of exon 11 that can allow alternative splicing between exons 10 and 12.

Close Modal
This Feature Is Available To Subscribers Only

or Create an Account

Close Modal
Close Modal