Dual expression of λ genes in the MOPC-315 plasmacytoma
The expression of two distinct κ light chain immunoglobulins in the MPC-11 mouse myeloma is well established 1–4 , the two protein products being apparently from RNA transcripts derived from separate, rearranged κ alleles in the MPC-11 genome 5–7 . Recently, the characterization of κ-related RNAs an...
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Veröffentlicht in: | Nature (London) 1981-03, Vol.290 (5801), p.65-67 |
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Zusammenfassung: | The expression of two distinct κ light chain immunoglobulins in the MPC-11 mouse myeloma is well established
1–4
, the two protein products being apparently from RNA transcripts derived from separate, rearranged κ alleles in the MPC-11 genome
5–7
. Recently, the characterization of κ-related RNAs and protein products In several λ-producing myelomas has indicated that multiple expression of light chain RNAs is a common event in myelomas and other cells of the B-lymphocyte lineage
5
. These studies suggest that, although many light chain alleles may function to make RNA and protein in a given B-lymphocytic cell, only one complete, functional light chain is generally translated from the RNAs present in a single cell. The myeloma, MOPC-315, synthesizes and secretes an antibody which has an α heavy chain and a λ
II
light chain
8
. The DNA of MOPC-315 either has no κ genes or has only a fragment of one, but it certainly has no κ genes in the embryonic configuration
5
. Rearrangement of its λ genes has been observed but the exact nature of the rearrangement is not known
9
. Because initial observations suggested that an immunoglobulin-related protein other than α and λ
II
was present in MOPC-315 cells
10
, we undertook to derive molecular cDNA clones from the mRNA in MOPC-315 tumour cells. Analysis of the clones has now identified two λ chain mRNA species: a normal Λ
II
chain mRNA and another which directs the synthesis of a deleted form of λ
I
protein. The nucleotide sequence of the deleted Λ
I
, mRNA shows that it resulted from a joining of the sequence encoding amino acid 31 of the variable region directly to the constant region coding sequence. |
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ISSN: | 0028-0836 1476-4687 |
DOI: | 10.1038/290065a0 |