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在盘基网柄菌中,与p110相关的PI 3激酶通过一条依赖蛋白激酶B/蛋白激酶B(PKB/Akt)的途径调节吞噬体-吞噬体融合及吞噬体pH值。

p110-related PI 3-kinases regulate phagosome-phagosome fusion and phagosomal pH through a PKB/Akt dependent pathway in Dictyostelium.

作者信息

Rupper A C, Rodriguez-Paris J M, Grove B D, Cardelli J A

机构信息

Department of Microbiology and Immunology, Louisiana State University Health Sciences Center, Shreveport, Louisiana 71130, USA.

出版信息

J Cell Sci. 2001 Apr;114(Pt 7):1283-95. doi: 10.1242/jcs.114.7.1283.

DOI:10.1242/jcs.114.7.1283
PMID:11256995
Abstract

The Dictyostelium p110-related PI 3-kinases, PIK1 and PIK2, regulate the endosomal pathway and the actin cytoskeleton, but do not significantly regulate internalization of particles in D. discoideum. Bacteria internalized into delta ddpik1/ddpik2 cells or cells treated with PI 3-kinase inhibitors remained intact as single particles in phagosomes with closely associated membranes after 2 hours of internalization, while in control cells, bacteria appeared degraded in multi-particle spacious phagosomes. Addition of LY294002 to control cells, after 60 minutes of chase, blocked formation of spacious phagosomes, suggesting PI 3-kinases acted late to regulate spacious phagosome formation. Phagosomes purified from control and drug treated cells contained equivalent levels of lysosomal proteins, including the proton pump complex, and were acidic, but in drug treated cells and delta ddpik1/ddpik2 cells phagosomal pH was significantly more acidic during maturation than the pH of control phagosomes. Inhibition of phagosomal maturation by LY294002 was overcome by increasing phagosomal pH with NH(4)Cl, suggesting that an increase in pH might trigger homotypic phagosome fusion. A pkbA null cell line (PKB/Akt) reproduced the phenotype described for cells treated with PI 3-kinase inhibitors and delta ddpik1/ddpik2 cells. We propose that PI 3-kinases, through a PKB/Akt dependent pathway, directly regulate homotypic fusion of single particle containing phagosomes to form multi-particle, spacious phagosomes, possibly through the regulation of phagosomal pH.

摘要

盘基网柄菌中与p110相关的PI 3激酶PIK1和PIK2调节内体途径和肌动蛋白细胞骨架,但对盘基网柄菌中颗粒的内化没有显著调节作用。内化2小时后,内化到缺失ddpik1/ddpik2的细胞或用PI 3激酶抑制剂处理的细胞中的细菌,作为单个颗粒完整地保留在膜紧密相连的吞噬体中,而在对照细胞中,细菌似乎在多颗粒的宽敞吞噬体中被降解。在追踪60分钟后,向对照细胞中添加LY294002可阻断宽敞吞噬体的形成,这表明PI 3激酶在后期发挥作用以调节宽敞吞噬体的形成。从对照细胞和药物处理细胞中纯化的吞噬体含有等量的溶酶体蛋白,包括质子泵复合物,并且呈酸性,但在药物处理细胞和缺失ddpik1/ddpik2的细胞中,吞噬体在成熟过程中的pH值比对照吞噬体的pH值酸性更强。用NH(4)Cl提高吞噬体pH值可克服LY294002对吞噬体成熟的抑制作用,这表明pH值的升高可能触发同型吞噬体融合。pkbA基因敲除细胞系(蛋白激酶B/蛋白激酶B)重现了用PI 3激酶抑制剂处理的细胞和缺失ddpik1/ddpik2的细胞所描述的表型。我们提出,PI 3激酶通过蛋白激酶B/蛋白激酶B依赖性途径,可能通过调节吞噬体pH值,直接调节含单个颗粒的吞噬体的同型融合,以形成多颗粒的宽敞吞噬体。

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