Mountz J D, Mushinski J F, Owens J D, Finkelman F D
Department of Medicine, University of Alabama, Birmingham 35294.
J Immunol. 1990 Sep 1;145(5):1583-91.
Mature, resting rodent, and primate B lymphocytes express two membrane Ig isotypes, IgM and IgD. Although membrane IgD production by these cells is regulated at a transcriptional level, and does not require deletion of the C mu gene, C mu has been deleted in all of the IgD-secreting tumor cells that have been studied. These IgD-secreting tumors, which include two mineral oil-induced plasmacytomas and three IgD-switch variants of an IgM-secreting hybridoma, might not, however, be representative of the rare IgD-secreting cells generated in response to an immune stimulus. A recent study of mice injected with a goat antibody to mouse IgD has demonstrated the generation of a relatively large secretory IgD response in these animals. We have now produced hybridomas by fusing spleen cells from these mice with a non-Ig-secreting plasmacytoma. Two of these hybridomas, KWD-1 and KWD-2, secrete IgD and express cell membrane IgD. Both of these hybridomas were found to have deleted the C mu gene. KWD-2 produces a delta-chain mRNA and a delta-chain protein similar in size to those previously reported for normal secreted mouse IgD; however, KWD-1 synthesizes a secretory delta-chain mRNA that is approximately 0.25 kb smaller than the KWD-2 secretory delta-chain mRNA and secretes IgD with a delta-chain that is approximately 21 kDa smaller than the secretory delta-chain of KWD-2. ELISA studies with epitope-defined anti-delta mAb indicate that KWD-2 has both delta Fc (C delta 3) [corrected] and delta Fd (C delta 1) [corrected] determinants, whereas KWD-1 has delta Fc but not delta Fd. These studies also demonstrate that the Ag-binding site of KWD-1 is not deleted because KWD-1 specifically binds goat IgG. Northern blot analyses with exon-specific probes indicate that while both KWD-1 and KWD-2 synthesize kappa-chain mRNA and delta-chain mRNA that includes the VH, C delta hinge, and C delta 3 exons, the C delta 1 exon is present only on the KWD-2 delta-chain mRNA. Southern blot analysis confirms that the C delta 1 exon has been deleted in KWD-1, but not KWD-2. We have previously noted that a secretory delta-chain mRNA that is similar in size to that produced by KWD-1 accounts for approximately 25% of the splenic secretory delta-chain mRNA produced by goat anti-mouse IgD antibody-injected mice.(ABSTRACT TRUNCATED AT 400 WORDS)
成熟的、静止的啮齿动物和灵长类B淋巴细胞表达两种膜免疫球蛋白(Ig)同种型,即IgM和IgD。尽管这些细胞产生膜IgD的过程在转录水平受到调控,且不需要删除Cμ基因,但在所有已研究的分泌IgD的肿瘤细胞中,Cμ基因均已缺失。然而,这些分泌IgD的肿瘤,包括两种矿物油诱导的浆细胞瘤和一种分泌IgM的杂交瘤的三种IgD转换变体,可能并不代表因免疫刺激而产生的罕见分泌IgD的细胞。最近一项对注射了抗小鼠IgD山羊抗体的小鼠的研究表明,这些动物产生了相对较大的分泌型IgD反应。我们现在通过将这些小鼠的脾细胞与一种不分泌Ig的浆细胞瘤融合,制备了杂交瘤。其中两种杂交瘤,KWD - 1和KWD - 2,分泌IgD并表达细胞膜IgD。发现这两种杂交瘤均缺失了Cμ基因。KWD - 2产生的δ链mRNA和δ链蛋白的大小与先前报道的正常分泌型小鼠IgD相似;然而,KWD - 1合成的分泌型δ链mRNA比KWD - 2的分泌型δ链mRNA小约0.25 kb,且分泌的IgD的δ链比KWD - 2的分泌型δ链小约21 kDa。用表位特异性抗δ单克隆抗体进行的ELISA研究表明,KWD - 2同时具有δFc(Cδ3)[校正后]和δFd(Cδ1)[校正后]决定簇,而KWD - 1具有δFc但不具有δFd。这些研究还表明,KWD - 1的抗原结合位点未被删除,因为KWD - 1能特异性结合山羊IgG。用外显子特异性探针进行的Northern印迹分析表明,虽然KWD - 1和KWD - 2都合成κ链mRNA和包含VH、Cδ铰链和Cδ3外显子的δ链mRNA,但Cδ1外显子仅存在于KWD - 2的δ链mRNA上。Southern印迹分析证实,KWD - 1中Cδ1外显子已缺失,而KWD - 2中未缺失。我们之前注意到,一种大小与KWD - 1产生的相似的分泌型δ链mRNA约占注射山羊抗小鼠IgD抗体的小鼠脾脏分泌型δ链mRNA的25%。(摘要截断于400字)
