Itoh Hiroshi, Kakuta Tomoko, Kudo Tetsuya, Sakonju Iwao, Hohdatsu Tsutomu, Ebina Takusaburo, Takase Katsuaki
Department of Veterinary Surgery, School of Veterinary Medicine and Animal Sciences, Kitasato University, Towada, Japan.
J Vet Med Sci. 2003 Mar;65(3):329-33. doi: 10.1292/jvms.65.329.
Interleukin (IL)-2 can induce large numbers of lymphokine-activated killer cells in peripheral blood lymphocytes (PBL), but IL-2 alone cannot induce proliferation of a large number of canine (c) PBL. We used the solid phase anti-CD3 antibody and soluble recombinant (r) IL-2 in order to establish a large scale culture method for cPBL. The number of lymphocytes seeded (3 x 10 (7)) increased to 1 x 10(9) after incubation for 10 days. The phenotype of cultured cPBL cells (after 2 weeks) showed a CD4(+) or CD8(+) predominant cell population. The cultured cell solutions were administered with physiological saline intravenously to each dog. After transfusion of the cultured cells, the cPBL counts, especially the number of CD4(+), CD8(+) and CD4(-)CD8 (-)(DN) cells increased significantly in the recipient dogs. Natural killer (NK) cells, gammadeltaT cells and B cells were considered to be present in the DN cell population. The NK cells and gammadeltaT cells showed no adverse reaction to the transfusion of the activated cPBL. Therefore, it is necessary to recognize the B cells present in the DN cell population by detecting CD21(+) cells. In conclusion, the bulk culture system of cPBL with rIL-2 and solid phase anti-CD3 antibody may be useful for the development of novel immunotherapy in dogs.
白细胞介素(IL)-2可在外周血淋巴细胞(PBL)中诱导产生大量淋巴因子激活的杀伤细胞,但单独的IL-2不能诱导大量犬(c)PBL增殖。我们使用固相抗CD3抗体和可溶性重组(r)IL-2来建立一种用于cPBL的大规模培养方法。接种的淋巴细胞数量(3×10⁷)在培养10天后增加到1×10⁹。培养的cPBL细胞(2周后)的表型显示为CD4⁺或CD8⁺为主的细胞群。将培养的细胞溶液用生理盐水静脉注射给每只狗。输入培养的细胞后,受体犬的cPBL计数,特别是CD4⁺、CD8⁺和CD4⁻CD8⁻(DN)细胞的数量显著增加。自然杀伤(NK)细胞、γδT细胞和B细胞被认为存在于DN细胞群中。NK细胞和γδT细胞对激活的cPBL的输入未显示不良反应。因此,有必要通过检测CD21⁺细胞来识别DN细胞群中存在的B细胞。总之,用rIL-2和固相抗CD3抗体进行cPBL的批量培养系统可能对犬新型免疫疗法的开发有用。
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