Fig. 6.
Fig. 6. Identification of 4.1R HE mutations. / (A) Identification of the genomic mutations by restriction digestion. In 4.1R Fier, the deletion neither creates nor abolishes a restriction site. (A1 + Ct) and (B1 + Ct) correspond to mixtures of patient and control DNAs. The restriction map is indicated at the bottom. Ct indicates control DNAs; and Mk, size markers. All sizes are in base pairs. (B) Reticulocyte 4.1R mRNA analysis. DdeI restriction digestion of RT-PCR product in 4.1R Fier revealed a single band that corresponds to the normal allele. In 4.1R Coimbra, RT-PCR amplification yielded 2 additional bands, CO.1 and CO.2, in the affected family members.

Identification of 4.1R HE mutations.

(A) Identification of the genomic mutations by restriction digestion. In 4.1R Fier, the deletion neither creates nor abolishes a restriction site. (A1 + Ct) and (B1 + Ct) correspond to mixtures of patient and control DNAs. The restriction map is indicated at the bottom. Ct indicates control DNAs; and Mk, size markers. All sizes are in base pairs. (B) Reticulocyte 4.1R mRNA analysis. DdeI restriction digestion of RT-PCR product in 4.1R Fier revealed a single band that corresponds to the normal allele. In 4.1R Coimbra, RT-PCR amplification yielded 2 additional bands, CO.1 and CO.2, in the affected family members.

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