Role of Adaptor Complex AP-3 in Targeting Wild-Type and Mutated CD63 to Lysosomes

Rous, Brian; Reaves, Barbara J.; Ihrke, Gudrun; Briggs, John; Gray, Sally R.; Stephens, David; Banting, George; Luzio, J. Paul

doi:10.1091/mbc.01-08-0409

Cited by 218 publications

(223 citation statements)

References 66 publications

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“…These results suggest that a significant pool of PI4KII␣ is controlled by the function of the adaptor complex AP-3. We note that PI4KII␣ was reported to interact with CD63 (Berditchevski et al, 1997;Yauch and Hemler, 2000), a membrane protein of lysosomes proposed to be sorted by AP-3-dependent mechanisms (Rous et al, 2002). Thus, it is possible that a direct or indirect interaction with CD63 may account, at least in part, for the localization of PI4KII␣ in AP-3-derived vesicles.…”

Section: Discussionmentioning

confidence: 82%

Phosphatidylinositol-4-Kinase Type II α Is a Component of Adaptor Protein-3-derived Vesicles

Salazar

Craige

Wainer

et al. 2005

MBoC

136

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A membrane fraction enriched in vesicles containing the adaptor protein (AP) -3 cargo zinc transporter 3 was generated from PC12 cells and was used to identify new components of these organelles by mass spectrometry. Proteins prominently represented in the fraction included AP-3 subunits, synaptic vesicle proteins, and lysosomal proteins known to be sorted in an AP-3-dependent way or to interact genetically with AP-3. A protein enriched in this fraction was phosphatidylinositol-4-kinase type II␣ (PI4KII␣). Biochemical, pharmacological, and morphological analyses supported the presence of PI4KII␣ in AP-3-positive organelles. Furthermore, the subcellular localization of PI4KII␣ was altered in cells from AP-3-deficient mocha mutant mice. The PI4KII␣ normally present both in perinuclear and peripheral organelles was substantially decreased in the peripheral membranes of AP-3-deficient mocha fibroblasts. In addition, as is the case for other proteins sorted in an AP-3-dependent way, PI4KII␣ content was strongly reduced in nerve terminals of mocha hippocampal mossy fibers. The functional relationship between AP-3 and PI4KII␣ was further explored by PI4KII␣ knockdown experiments. Reduction of the cellular content of PI4KII␣ strongly decreased the punctate distribution of AP-3 observed in PC12 cells. These results indicate that PI4KII␣ is present on AP-3 organelles where it regulates AP-3 function. INTRODUCTIONMembrane-enclosed organelles possess distinctive protein compositions that are dynamically maintained by inbound and outbound vesicle carriers. These vesicles selectively concentrate appropriate membrane proteins while leaving behind resident proteins found in the donor organelle, a process called sorting (Bonifacino and Glick, 2004). Central to membrane protein sorting and vesiculation are a family of cytosolic coat complexes that mediate vesicle budding and function as cargo-specific adaptors. These include monomeric proteins and the heterotetrameric adaptor proteins (AP)-1, -2, -3, and -4 (Bonifacino and Glick, 2004;Robinson, 2004). These coats participate in the generation of vesicles that carry a unique array of membrane protein "cargoes." The characterization of these carriers has played a major role in the functional dissection of coat-dependent sorting and vesiculation mechanisms. For example, vesicles "in a basket" isolated from brain led to the biochemical identification of the first sorting machinery, clathrin and the AP-1 and AP-2 adaptors (Kanaseki and Kadota, 1969;Pearse, 1975;Pfeffer and Kelly, 1981;Pearse and Crowther, 1987). Subsequent studies of cargo molecules in brain clathrin-coated vesicles were crucial in revealing mechanisms of synaptic vesicle recycling (Pfeffer and Kelly, 1985;Maycox et al., 1992;Blondeau et al., 2004). The advent of complete genome sequencing and the concomitant development of informatics tools has led to the rapid identification of proteins by mass spectrometry (Taylor et al., 2003). Application of these methodologies to clathrin-coated vesicles has allowed the identifi...

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Section: Discussionmentioning

confidence: 82%

Phosphatidylinositol-4-Kinase Type II α Is a Component of Adaptor Protein-3-derived Vesicles

Salazar

Craige

Wainer

et al. 2005

MBoC

136

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“…Previous work had shown that OCRL localizes to endosomes and the TGN (Ungewickell et al, 2004;Lowe, 2005). CVAK104 overlapped also significantly with the adaptor protein complex AP3, which is involved in the sorting of lysosomal membrane proteins (Le Borgne et al, 1998;Rous et al, 2002) (Figure 4C). In contrast, very little colocalization of CVAK104 with early endosomal markers such as early endosomal antigen (EEA)1 ( Figure 4C) and rab5 (our unpublished data) was seen.…”

Section: Tissue Expression and Subcellular Localization Of Cvak104mentioning

confidence: 74%

Clathrin-dependent Association of CVAK104 with Endosomes and theTrans-Golgi Network

Düwel

Ungewickell

2006

MBoC

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“…20 Therefore, we hypothesized that NE precursor (proNE) is routed to granules through the protein-delivery pathway of CD63, which recruits AP-3 adaptor complex through the C-terminal lysosomal targeting motif GYEVM. 21 Thus, cooperation with CD63 was thought to facilitate the secretory lysosome targeting of proNE.To corroborate our hypothesis, we examined whether CD63 and proNE interacted upon coexpression in COS cells. Furthermore, we examined how CD63 depletion affected proNE trafficking.…”

mentioning

confidence: 74%

“…The CD63AEVM mutant has a single amino acid mutation in the C-terminal lysosomal sorting sequence that decreases intracellular CD63 and plasma membrane sorting. 21 Although not formally proved, CD63AEVM might produce nonfunctional complexes that are likely to be degraded or become transferred to the plasma membrane.In the 5 clones investigated, CD63 siRNA expression showed a mean of 6.5-fold (the range was from 16-fold to 3.7-fold) suppression of CD63 mRNA compared with wild-type cells, CD63 siRNA mock, or a reverted CD63siRNA clone ( Figure 5A). The CD63 mRNA levels of 5 cell clones with scrambled siRNA control vector did not differ from wild-type cells ( Figure S2A).…”

mentioning

confidence: 99%

The tetraspanin CD63 is involved in granule targeting of neutrophil elastase

Källquist

Hansson

Persson

et al. 2008

Blood

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Targeting mechanisms of neutrophil elastase (NE) and other luminal proteins stored in myeloperoxidase (MPO)-positive secretory lysosomes/primary granules of neutrophils are unknown. These granules contain an integral membrane protein, CD63, with an adaptor protein-3-dependent granule delivery system. Therefore, we hypothesized that CD63 cooperates in granule delivery of the precursor of NE (proNE). Supporting this hypothesis, an association was demonstrated between CD63 and proNE upon coexpression in COS cells. This also involved augmented cellular retention of proNE requiring intact large extracellular loop of CD63. Furthermore, depletion of CD63 in promyelocytic HL-60 cells with RNA interference or a CD63 mutant caused reduction of cellular NE. However, the proNE steady-state level was similar to wild type in CD63-depleted clones, making it feasible to examine possible effects of CD63 on NE trafficking. Thus, depletion of CD63 led to reduced processing of proNE into mature NE and reduced constitutive secretion. Furthermore, CD63-depleted cells showed a lack of morphologically normal granules, but contained MPO-positive cytoplasmic vacuoles with a lack of proNE and NE. Collectively, our data suggest that granule proteins may cooperate in targeting; CD63 can be involved in ER or Golgi export, cellular retention, and granule targeting of proNE before storage as mature NE. (Blood. 2008;112:3444-3454) IntroductionHematopoietic cells play a critical role in host defense, for which they are equipped with secretory lysosomes or lysosome-related organelles that can release cell-specific cytolytic proteins by regulated secretion. 1,2 The secretory lysosomes/primary granules of neutrophils are furnished with an array of proteins that includes hematopoietic serine proteases along with myeloperoxidase (MPO), other microbicidal proteins, and specific transmembrane proteins. 3,4 The precise functions of the hematopoietic serine proteases-neutrophil elastase (NE), cathepsin G, proteinase 3, and azurocidin-are not fully known, but all 4 are thought to be important in the innate immunity function provided by neutrophils. 5,6 These proteases are synthesized as transient proforms that become catalytically active (except for azurocidin) by removal of an N-terminal propeptide after granule targeting. 7,8 Lysosome hydrolases and granzymes use a mannose-6-phosphate (MP) signal and binding to an MP receptor for targeting, 9,10 but the signals for the targeting of hematopoietic serine proteases are not yet known. Cargo proteins can be transported to secretory lysosomes independent of the MP system, 11 as is illustrated by the fact that in I-cell disease, neutrophils and other cells have a normal content of hydrolases despite a lack of MP synthesis. 12 The delivery of a soluble protein might occur through the assistance of a cooperating transmembrane partner that establishes contact with adaptor proteins (APs) to recruit the transport system necessary for targeting. The adaptor protein AP-3 is known to have a role in bringing transmembr...

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Role of Adaptor Complex AP-3 in Targeting Wild-Type and Mutated CD63 to Lysosomes

Cited by 218 publications

References 66 publications

Phosphatidylinositol-4-Kinase Type II α Is a Component of Adaptor Protein-3-derived Vesicles

Phosphatidylinositol-4-Kinase Type II α Is a Component of Adaptor Protein-3-derived Vesicles

Clathrin-dependent Association of CVAK104 with Endosomes and theTrans-Golgi Network

The tetraspanin CD63 is involved in granule targeting of neutrophil elastase

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