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P2Z-Independent and P2Z Receptor-Mediated Macrophage Killing by Pseudomonas aeruginosa Isolated from Cystic Fibrosis Patients

机译:囊性纤维化患者分离的铜绿假单胞菌的P2Z独立和P2Z受体介导的巨噬细胞杀伤。

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摘要

We demonstrate that a mucoid, alginate-producing strain of Pseudomonas aeruginosa isolated from the lungs of a cystic fibrosis (CF) patient secretes multiple enzymes with nucleoside diphosphate kinase (Ndk), ATPase, adenylate kinase, 5′-nucleotidase, and ATP-modifying enzymatic activities. The secretion is triggered at high cell density and in complex media but is greatly reduced when the mucoid cells are grown in mineral salts media or in presence of 5.0 mM Ca2+ or Mg2+. Interestingly, the secretion is triggered primarily in the mucoid CF isolate of strain 8821M (or in strain FRD1) but not in a nonmucoid laboratory strain, PAO1. The purified secreted Ndk shows 100% match in its N-terminal amino acid sequence with that of purified intracellular Ndk and demonstrates similar enzymatic properties. The N-terminal sequence of the purified ATPase isolated from an ndk knockout mutant shows its identity with that of the heat shock chaperonin Hsp60. During fractionation, the flowthrough fraction from a Mono Q column demonstrates the presence of 5′-nucleotidase, adenylate kinase, and a putative ATP reductase activity. These fractions demonstrate high cytotoxic activities for murine peritoneal primary macrophages which can be further stimulated in the presence of ATP or inhibited by pretreatment of macrophages with oxidized ATP (oATP). The cytotoxicity associated with ATP-induced stimulation is believed to be due to activation of macrophage surface-associated P2Z (P2X7) receptors, which are one of the purinergic receptors responsible for pore formation on macrophage membrane. Blocking of these receptors by pretreatment with oATP blocks ATP-induced macrophage cell death. Thus mucoid P. aeruginosa cells elaborate enzymes that modulate the external ATP levels of macrophages, thereby modulating macrophage cell death through P2Z receptor activation. Evidence for the presence of secreted cytotoxic agents that act independently of P2Z receptor activation is also presented.
机译:我们证明,从囊性纤维化(CF)患者的肺中分离出的铜绿假单胞菌的粘液样藻酸盐生产菌株分泌多种酶与核苷二磷酸激酶(Ndk),ATPase,腺苷酸激酶,5'-核苷酸酶和ATP修饰酶促活动。分泌是在高细胞密度和复杂培养基中触发的,但是当粘液状细胞在矿物盐培养基中或在5.0 mM Ca 2 + 或Mg 2+ < / sup>。有趣的是,分泌主要在菌株8821M的粘液CF分离株中(或在FRD1菌株中)触发,而不是在非粘液实验室菌株PAO1中触发。纯化的分泌的Ndk在其N末端氨基酸序列中与纯化的细胞内Ndk的氨基酸序列显示100%匹配,并显示出相似的酶促性质。从ndk基因敲除突变体中分离出的纯化ATPase的N末端序列与热激伴侣蛋白Hsp60的N末端序列具有同一性。在分馏过程中,来自Mono Q色谱柱的流通级分证明存在5'-核苷酸酶,腺苷酸激酶和假定的ATP还原酶活性。这些级分显示出对鼠腹膜原代巨噬细胞的高细胞毒性活性,可在ATP存在下进一步刺激或通过用氧化ATP(oATP)预处理巨噬细胞来抑制这种抑制作用。据信与ATP诱导的刺激相关的细胞毒性是由于巨噬细胞表面相关的P2Z(P2X7)受体的激活所致,P2Z(P2X7)受体是负责在巨噬细胞膜上形成孔的嘌呤能受体之一。通过用oATP预处理阻断这些受体可阻断ATP诱导的巨噬细胞死亡。因此,粘液铜绿假单胞菌细胞精心制作了可调节巨噬细胞外部ATP水平的酶,从而可通过P2Z受体激活来调节巨噬细胞死亡。还提供了存在与P2Z受体激活无关的分泌细胞毒剂的证据。

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