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Showing papers by "Shizuo Akira published in 1983"


Journal ArticleDOI
01 Sep 1983-Cell
TL;DR: The results showed that isotype switching can operate at the stage of pre-B cells by a CH gene deletion mechanism without utilizing the switch region, and the possibility is presented that deletion of the intervening CH genes could occur prior to the formation of the functional V region-coding DNA segment.

50 citations


Journal ArticleDOI
30 Jun 1983-Nature
TL;DR: Southern blot analysis of the DNA and two-dimensional gel electrophoresis of intracytoplasmic μ-chain show thatμ-chain diversity with respect to antigen specificity may be generated during this second rearrangement process, and implies that light-chain gene rearrangements requires some further change, or a different enzyme.
Abstract: B lymphocytes originate from pluripotential haematopoietic stem cells and differentiate into immunoglobulin (Ig)-producing cells. B-cell lineage differentiation is accompanied by two types of immunoglobulin gene rearrangements--rearrangement of V, D and J gene segments to create a functional V gene and rearrangement of CH genes for heavy-chain switching. These results, however, have been obtained mainly by analysis of immunoglobulin gene organization of myeloma cells. Baltimore and his colleagues have established Abelson murine leukaemia virus (A-MuLV)-transformed cell lines and found a few lines capable of carrying out kappa-gene rearrangement or undergoing isotype switching during in vitro culture. To study early B-cell lineage differentiation events, we have now also established A-MuLV-transformed cell lines which are capable of differentiating from mu- to mu+ and of undergoing continuing rearrangement of heavy-chain genes in culture. Analysis of immunoglobulin gene organization of these transformed cells revealed that mu- cells have already undergone DNA rearrangements involving JH segments but an additional rearrangement of JH segments is required for initiation of mu-chain synthesis. Southern blot analysis of the DNA and two-dimensional gel electrophoresis of intracytoplasmic mu-chain show that mu-chain diversity with respect to antigen specificity may be generated during this second rearrangement process. As no rearrangement of light-chain genes takes place in these cells, this implies that light-chain gene rearrangement requires some further change, or a different enzyme.

44 citations