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多糖制剂PSK在体外可增强肿瘤浸润淋巴细胞的增殖和细胞毒性。

Polysaccharide preparation PSK augments the proliferation and cytotoxicity of tumor-infiltrating lymphocytes in vitro.

作者信息

Noguchi K, Tanimura H, Yamaue H, Tsunoda T, Iwahashi M, Tani M, Mizobata S, Hotta T, Arii K, Tamai M

机构信息

Department of Gastroenterological Surgery, Wakayama Medical School, Japan.

出版信息

Anticancer Res. 1995 Mar-Apr;15(2):255-8.

PMID:7762991
Abstract

We have investigated whether or not polysaccharide preparation PSK directly augments the proliferation and cytotoxicity of tumor-infiltrating lymphocytes (TILs). TILs were separated from 10 patients with gastrointestinal cancer (5 gastric cancers, 3 colon cancers and 2 pancreatic cancers). TILs were cultured with IL-2 and PSK for 7 days. The DNA synthesis of TILs was augmented by incubation with 100 micrograms/ml of PSK, which was similar to serum level with oral administration of PSK in cancer patients. The effect of PSK in DNA synthesis was also found by elimination of non-T cells. Furthermore, we established TIL clones and examined the effect of PSK on TILs clones. The DNA synthesis was augmented by PSK in CD4 positive and CD8 positive TIL clones without non-T cells, suggesting that PSK acts directly on TILs. We examined the cytotoxic activities of TILs by the 4-h and 16-h 51Cr release assay. PSK did not affect the cytotoxic activity of TILs against autologous tumor cells and KATO-III cells in the 4h 51Cr release assay, whereas PSK induced high lysability of TILs against autologous tumor cells in the 16-h 51Cr release assay. We studied the ability of PSK to induce cytokines from TILs using a double chamber plate. The DNA synthesis of tumor cells was more suppressed by the mixed-tumor cell culture supernatants of TILs cultured with PSK, compared to that of TILs cultured without PSK. It is suggesting that PSK induced long term killing activity of TILs by induction of cytotoxic cytokines. Thus, PSK augmented the proliferative response of TILs without interaction of T cells and non-T cells and induced cytotoxic cytokines of TILs.

摘要

我们研究了多糖制剂PSK是否能直接增强肿瘤浸润淋巴细胞(TILs)的增殖和细胞毒性。从10例胃肠道癌患者(5例胃癌、3例结肠癌和2例胰腺癌)中分离出TILs。将TILs与白细胞介素-2(IL-2)和PSK一起培养7天。用100微克/毫升的PSK孵育可增强TILs的DNA合成,这与癌症患者口服PSK时的血清水平相似。通过去除非T细胞也发现了PSK在DNA合成中的作用。此外,我们建立了TIL克隆,并检测了PSK对TIL克隆的影响。在没有非T细胞的CD4阳性和CD8阳性TIL克隆中,PSK增强了DNA合成,这表明PSK直接作用于TILs。我们通过4小时和16小时的51铬释放试验检测了TILs的细胞毒性活性。在4小时51铬释放试验中,PSK不影响TILs对自体肿瘤细胞和KATO-III细胞的细胞毒性活性,而在16小时51铬释放试验中,PSK诱导TILs对自体肿瘤细胞具有高裂解性。我们使用双室板研究了PSK诱导TILs产生细胞因子的能力。与未用PSK培养的TILs相比,用PSK培养的TILs的混合肿瘤细胞培养上清液对肿瘤细胞DNA合成的抑制作用更强。这表明PSK通过诱导细胞毒性细胞因子诱导TILs产生长期杀伤活性。因此,PSK增强了TILs的增殖反应,而无需T细胞和非T细胞的相互作用,并诱导了TILs的细胞毒性细胞因子。

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