Okura Eiji, Ishimaru Aiko, Yamamoto Aki, Nakatsu Shino, Shirakura Ryota, Okabe Masaru, Sawa Yoshiki, Fukuzawa Masahiro, Okumura Meinoshin, Miyagawa Shuji
Division of Organ Transplantation, Department of Molecular Therapeutics, Osaka University Graduate School of Medicine, Suita, Osaka, Japan.
Xenotransplantation. 2008 Nov-Dec;15(6):365-73. doi: 10.1111/j.1399-3089.2008.00496.x.
Expression of complement regulatory proteins (CRP) on pig endothelial cells (PEC) is an effective means of avoiding induction of hyperacute rejection by human sera. However, pig endogenous retrovirus (PERV) from PEC transfected with CRP may acquire resistance to human sera. This study investigated a form of transfected CRP that is easily expressed on PERV particles.
The PEC line was transfected with the Lac Z gene and PERV-B to investigate PERV infectivity using a Lac Z pseudo-type assay. The cDNAs of several modified DAF (CD55) were then transfected into the PEC(Lac Z)/P-B lines using lipofection. DAF expression was verified by FACS analysis. Complement-dependent PEC lysis was tested to verify the complement regulatory function of the expressed DAF. HEK293 cells were incubated with PEC culture supernatants with or without human sera. The inoculated 293 cells were histochemically stained and Lac Z-positive blue foci were counted. The rate of reduction in Lac Z-positive cells resulting from the addition of human serum was then calculated. In addition, to assess the localization of the expressed DAF, flotation sucrose density analysis was performed.
While PERV released from PEC expressing delta-short consensus repeat 2 (delta-SCR2) DAF (lacking CRP function) showed no change in resistance to human serum compared to control cells, PERV from cells expressing delta-SCR1 DAF (with CRP function) showed a significant increase in resistance. The DAF-blocking antibody assay indicated that PERV from the DAF transfectants expressed DAF molecules on the surface of the retrovirus. While delta-SCR1 DAF (PI-anchor form) significantly inhibited the reduction of Lac Z-positive cells by human serum, the reduction of Lac Z-positive cells by human serum was less inhibited in the case of transmembrane (TM)-types of DAF-HLA-G, modified influenza hemagglutinin (HA) and MCP (delta-CYT form). However, the reduction in each TM-type DAF was slightly less than that observed in naive and mock cells. The flotation sucrose density analysis of these transfectants indicated that the PI-anchor form of DAF is a raft-associated protein, and most TM-types of DAF are non-raft proteins.
Induction of resistance to human serum in PERV, depends on the form of the CRP tail. The CRP/TM hybrid that does not associate with lipid rafts, is a suitable form of CRP for gene transduction.
猪内皮细胞(PEC)上补体调节蛋白(CRP)的表达是避免人血清诱导超急性排斥反应的有效手段。然而,转染了CRP的PEC中的猪内源性逆转录病毒(PERV)可能会获得对人血清的抗性。本研究调查了一种易于在PERV颗粒上表达的转染CRP形式。
用Lac Z基因和PERV - B转染PEC系,使用Lac Z假型试验研究PERV的感染性。然后用脂质体转染法将几种修饰的衰变加速因子(CD55)的cDNA转染到PEC(Lac Z)/P - B系中。通过流式细胞术分析验证DAF的表达。测试补体依赖性PEC裂解以验证表达的DAF的补体调节功能。将HEK293细胞与含或不含人血清的PEC培养上清液孵育。对接种的293细胞进行组织化学染色并计数Lac Z阳性蓝色斑点。然后计算加入人血清导致的Lac Z阳性细胞减少率。此外,为了评估表达的DAF的定位,进行了浮选蔗糖密度分析。
与对照细胞相比,从表达δ - 短共有重复序列2(δ - SCR2)DAF(缺乏CRP功能)的PEC释放的PERV对人血清的抗性没有变化,而从表达δ - SCR1 DAF(具有CRP功能)的细胞释放的PERV抗性显著增加。DAF阻断抗体试验表明,来自DAF转染体的PERV在逆转录病毒表面表达DAF分子。虽然δ - SCR1 DAF(PI - 锚定形式)显著抑制人血清对Lac Z阳性细胞的减少,但对于跨膜(TM)型的DAF - HLA - G、修饰的流感血凝素(HA)和膜辅蛋白(MCP,δ - CYT形式),人血清对Lac Z阳性细胞的减少抑制作用较小。然而,每种TM型DAF的减少略低于未处理细胞和模拟细胞中的观察值。这些转染体的浮选蔗糖密度分析表明,DAF的PI - 锚定形式是一种与脂筏相关的蛋白质,大多数TM型DAF是非脂筏蛋白质。
PERV中对人血清抗性的诱导取决于CRP尾部的形式。不与脂筏相关的CRP/TM杂合体是一种适合基因转导的CRP形式。
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