Marenne Marie-Noëlle, Journet Laure, Mota Luis Jaime, Cornelis Guy R
Christian de Duve Institute of Cellular Pathology and Faculté de Médecine, Université de Louvain, B-1200, Brussels, Belgium.
Microb Pathog. 2003 Dec;35(6):243-58. doi: 10.1016/s0882-4010(03)00154-2.
The Ysc-Yop type III secretion (TTS) system allows extracellular Yersinia bacteria, adhering to eukaryotic target cells, to inject Yop effector proteins in the cytosol of these cells. The secretion apparatus, called the injectisome, ends up with a needle-like structure made of YscF. YopN, one of the proteins secreted by the injectisome is thought to act as a plug. YopB, YopD and LcrV, three other proteins secreted by the injectisome and called 'translocators' form a pore allowing translocation of the Yop effectors across the target cell plasma membrane. Here, we tested the role of LcrV, YscF and YopN in the formation of this pore in macrophages by monitoring the release of the low-molecular-weight fluorescent dye BCECF (2',7'-bis-(2-carboxyethyl)-5-(and-6)-carboxyfluorescein, acetoxymethyl ester, 623Da) and of the high-molecular-weight lactate dehydrogenase (LDH, 135 kDa). BCECF is released through the translocation pore itself provided no Yop effector is trafficking through the channel. In contrast, LDH is released by the osmotic lysis of the target cell that occurs after pore formation. This release is reduced by the GAP activity of YopE. In order to study the role of LcrV, one has to circumvent the regulatory effect of LcrV on the synthesis of YopB and YopD. We observed here that this regulatory role of LcrV is lost in a yopQ mutant and hence we studied the role of LcrV in a yopQ mutant background. A lcrV, yopQ double mutant was deficient in pore formation while able to produce YopB and YopD. Pore formation was restored by the introduction of lcrV(+) but not yopQ(+) confirming that LcrV itself is directly required for pore formation. Bacteria secreting only YopB, YopD and LcrV could form pores, showing that YopB, YopD and LcrV are sufficient for pore formation provided they are secreted by the same bacterium. LcrV is not involved in secretion of YopB and YopD as suggested previously. Bacteria producing normal Ysc injectisomes, including the YscF needle but no translocators did not form pores, indicating that the needle is not sufficient by itself for pore formation, as was also suggested. yopN mutant bacteria formed needles and released BCECF even if they secreted the effectors. This observation suggests that many translocation pores are not filled in the absence of YopN and thus that YopN might form a link between the needle and the pore, guiding the effectors.
Ysc-Yop III型分泌(TTS)系统使附着于真核靶细胞的细胞外耶尔森氏菌能够将Yop效应蛋白注入这些细胞的胞质溶胶中。这种分泌装置称为注射体,最终形成由YscF构成的针状结构。注射体分泌的蛋白之一YopN被认为起到塞子的作用。注射体分泌的另外三种蛋白YopB、YopD和LcrV被称为“转运体”,它们形成一个孔,使Yop效应蛋白能够穿过靶细胞质膜进行转运。在此,我们通过监测低分子量荧光染料BCECF(2',7'-双(2-羧乙基)-5-(和-6)-羧基荧光素,乙酰氧基甲酯,623Da)和高分子量乳酸脱氢酶(LDH,135kDa)的释放,测试了LcrV、YscF和YopN在巨噬细胞中该孔形成过程中的作用。如果没有Yop效应蛋白通过通道转运,BCECF会通过转运孔本身释放出来。相反,LDH是在孔形成后靶细胞发生渗透性裂解而释放的。YopE的GAP活性会减少这种释放。为了研究LcrV的作用,必须规避LcrV对YopB和YopD合成的调节作用。我们在此观察到,LcrV的这种调节作用在yopQ突变体中丧失,因此我们在yopQ突变体背景下研究了LcrV的作用。lcrV、yopQ双突变体在孔形成方面存在缺陷,但其能够产生YopB和YopD。通过导入lcrV(+)而非yopQ(+)可恢复孔的形成,这证实LcrV本身是孔形成直接所需的。仅分泌YopB、YopD和LcrV的细菌能够形成孔,这表明只要YopB、YopD和LcrV由同一细菌分泌,它们就足以形成孔。LcrV并不像先前认为的那样参与YopB和YopD的分泌。产生正常Ysc注射体(包括YscF针但没有转运体)的细菌不能形成孔,这表明针本身不足以形成孔,这一点也已被提及。yopN突变体细菌即使分泌效应蛋白也能形成针并释放BCECF。这一观察结果表明,在没有YopN的情况下,许多转运孔并未被填满,因此YopN可能在针和孔之间形成连接,引导效应蛋白。
