Figure 4
Figure 4. Identification of the polyA addition site of the APH-2 transcript. (A) RNA samples obtained from 293T cells transfected with the pHTLV-2 ΔEcoRI plasmid (lane 2) were analyzed by 3′ RLM-RACE using the 21-3 primer. Lane 1 represents PCR amplification in the absence of any cDNA. M indicates 100-bp marker. (B) Position of the polyA addition site next to a consensus polyA signal and a GT-rich consensus sequence. The sequences of the APH-2 mRNA and of the 3′ polyA tail are shown. ■ represents the coding portion of the APH-2 spliced transcript. HTLV-2 sequences retrieved from GenBank were also compared using MO as a reference sequence. Comparisons were focused on the AATAAA polyA signal (position 5185 on the sense strand), the cleavage site deduced from our 3′RACE results and the GT-rich sequence. (C) PolyA+ RNA was extracted from pHTLV-2 ΔEcoRI-transfected 293T cells (lane 1) or from nontransfected cells (lane 2) and was run on a 1.5% agarose gel. After migration and transfer, the membrane was hybridized with a probe corresponding to the coding segment of the APH-2 cDNA and signals were revealed with a PhosphorImager. An RNA marker was migrated in parallel and corresponding molecular weights are indicated on the left side of the panel.

Identification of the polyA addition site of the APH-2 transcript. (A) RNA samples obtained from 293T cells transfected with the pHTLV-2 ΔEcoRI plasmid (lane 2) were analyzed by 3′ RLM-RACE using the 21-3 primer. Lane 1 represents PCR amplification in the absence of any cDNA. M indicates 100-bp marker. (B) Position of the polyA addition site next to a consensus polyA signal and a GT-rich consensus sequence. The sequences of the APH-2 mRNA and of the 3′ polyA tail are shown. ■ represents the coding portion of the APH-2 spliced transcript. HTLV-2 sequences retrieved from GenBank were also compared using MO as a reference sequence. Comparisons were focused on the AATAAA polyA signal (position 5185 on the sense strand), the cleavage site deduced from our 3′RACE results and the GT-rich sequence. (C) PolyA+ RNA was extracted from pHTLV-2 ΔEcoRI-transfected 293T cells (lane 1) or from nontransfected cells (lane 2) and was run on a 1.5% agarose gel. After migration and transfer, the membrane was hybridized with a probe corresponding to the coding segment of the APH-2 cDNA and signals were revealed with a PhosphorImager. An RNA marker was migrated in parallel and corresponding molecular weights are indicated on the left side of the panel.

Close Modal
This Feature Is Available To Subscribers Only

or Create an Account

Close Modal
Close Modal