Fig. 3.
Fig. 3. Comparison of B-cell and plasma cell RHAMM. RHAMM cDNA fragments were amplified from MM B cells and BM plasma cells by RT-PCR with RHAMM-specific primers and subsequently cloned and sequenced. The nucleotide sequences of the RHAMM fragments were aligned to generate the sequence of B-cell RHAMMFL and BM plasma cell RHAMMFL. The 48-bp deletion and the 147-bp deletion that characterize RHAMM−48 and RHAMM−147,respectively, are marked in bold lowercase. The 2 ATG start codons (base 18-20 and base 363-365) and TAA stop codon (base 2197-2199), previously described for breast RHAMM, plus the 2 HA-binding domains are underlined.

Comparison of B-cell and plasma cell RHAMM. RHAMM cDNA fragments were amplified from MM B cells and BM plasma cells by RT-PCR with RHAMM-specific primers and subsequently cloned and sequenced. The nucleotide sequences of the RHAMM fragments were aligned to generate the sequence of B-cell RHAMMFL and BM plasma cell RHAMMFL. The 48-bp deletion and the 147-bp deletion that characterize RHAMM−48 and RHAMM−147,respectively, are marked in bold lowercase. The 2 ATG start codons (base 18-20 and base 363-365) and TAA stop codon (base 2197-2199), previously described for breast RHAMM, plus the 2 HA-binding domains are underlined.

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