Exocyst Is Involved in Cystogenesis and Tubulogenesis and Acts by Modulating Synthesis and Delivery of Basolateral Plasma Membrane and Secretory Proteins

Lipschutz, Joshua H.; Guo, Wei; O’Brien, Lucy Erin; Nguyen, Yen; Novick, Peter; Mostov, Keith E.

doi:10.1091/mbc.11.12.4259

Cited by 146 publications

(182 citation statements)

References 91 publications

(92 reference statements)

Supporting

Mentioning

167

Contrasting

Order By: Relevance

“…Branching morphogenesis of tubular epithelium is a common and important feature of vertebrate organogenesis [1,22,32]. The MAPK/ERK pathway, which is downstream of receptor tyrosine kinases, leads to the phosphorylation, and hence activation, of ERK and has been shown to be important in branching morphogenesis in several systems, including the Drosophila trachea [20] and murine salivary gland [21].…”

Section: Discussionmentioning

confidence: 99%

“…Recombinant HGF at 100 ng/ml was added to the basolateral compartment of MDCK cell monolayers following a 1 h pretreatment either with or without U0126 (Promega) or PD098059 (Sigma), both inhibitors of MEK, at 10 μM and 50μM respectively. HGF at 100 ng/ml has been shown to induce tubulogenesis in MDCK cells [1,19]. Recombinant human HGF was generously provided by the late R. Schwall (Genentech, South San Francisco).…”

Section: Mdck Culture Hgf Treatment and Rna Isolationmentioning

confidence: 99%

“…Epithelial organs such as the kidney, lung, and salivary gland develop from a process termed branching morphogenesis [1]. Though branching morphogenesis is incompletely understood, genes involved in this process are conserved in different organs, and indeed throughout evolution.…”

Section: Introductionmentioning

confidence: 99%

“…The vast majority of studies examining cyst and tubule formation using MDCK cells were performed with Strain II cells [1,11,12]. MDCK Strain I cells, derived from an early passage of the cell population, and MDCK Strain II cells, which predominate in later passages, originated from separate nephron segments [13,14].…”

Section: Introductionmentioning

confidence: 99%

See 3 more Smart Citations

Intracellular signaling via ERK/MAPK completes the pathway for tubulogenic fibronectin in MDCK cells

Zhao

Greco

Hellman

et al. 2007

Biochemical and Biophysical Research Communications

Self Cite

View full text Add to dashboard Cite

A classic in vitro model of branching morphogenesis utilizes the Madin-Darby canine kidney (MDCK) cell line. MDCK Strain II cells form hollow monoclonal cysts in a three-dimensional collagen matrix over the course of ten days and tubulate in response to hepatocyte growth factor (HGF). We and our colleagues previously showed that activation of the extracellular-signal regulated kinase (ERK, aka MAPK) pathway is necessary and sufficient to induce tubulogenesis in MDCK cells. We also showed in a microarray study that one of the genes upregulated by HGF was the known tubulogene fibronectin. Given that HGF activates a multitude of signaling pathways, including ERK/ MAPK, to test the intracellular regulatory pathway, we used two distinct inhibitors of ERK activation (U0126 and PD098059). Following induction of MDCK Type II cells with HGF, tubulogenic fibronectin mRNA was upregulated 4-fold by real time PCR, and minimal or no change in fibronectin expression was seen when HGF was added with either U0126 or PD098059. We confirmed these results using an MDCK cell line inducible for Raf, which is upstream of ERK. Following activation of Raf, fibronectin mRNA and protein expression were increased to a similar degree as was seen following HGF induction. Furthermore, MDCK Strain I cells, which originate from collecting ducts and have constitutively active ERK, spontaneously initiate tubulogenesis. We show here that MDCK Strain I cells have high levels of fibronectin mRNA and protein compared to MDCK Strain II cells. When U0126 and PD098059 were added to MDCK Strain I cells, fibronectin mRNA and protein levels were decreased to levels seen in MDCK Strain II cells. These data allow us to complete what we believe is the first description of a tubulogenic pathway from receptor/ligand (HGF/CMET), through an intracellular signaling pathway (ERK/MAPK), to transcription and, finally, secretion of a critical tubuloprotein (fibronectin).

show abstract

Section: Discussionmentioning

confidence: 99%

Section: Mdck Culture Hgf Treatment and Rna Isolationmentioning

confidence: 99%

Section: Introductionmentioning

confidence: 99%

Section: Introductionmentioning

confidence: 99%

See 2 more Smart Citations

Intracellular signaling via ERK/MAPK completes the pathway for tubulogenic fibronectin in MDCK cells

Zhao

Greco

Hellman

et al. 2007

Biochemical and Biophysical Research Communications

Self Cite

View full text Add to dashboard Cite

show abstract

“…LDLR fusion was shown at this site by time-lapse confocal microscopy (Kreitzer et al, 2003), and Shrew-1 and VSV-G fusion was found at this site by tannic acid-blocking experiments (Polishchuk et al, 2004;Jakob et al, 2006). In polarized MDCK cells, the Sec6/8 complex is recruited to (Yeaman et al, 2004) and localized at the apical junctional complex along the lateral membrane (Grindstaff et al, 1998;Lipschutz et al, 2000), which is recognized to be an area of active exocytosis (Kreitzer et al, 2003). We previously reported that Naked2-associated vesicles accumulated asymmetrically at the basolateral corner of MDCK cells stably expressing myristoylation-deficient G2A Naked2.…”

Section: Naked2-coated Vesicles Target Initially To the Lower Portionmentioning

confidence: 95%

Naked2 Acts as a Cargo Recognition and Targeting Protein to Ensure Proper Delivery and Fusion of TGF-α–containing Exocytic Vesicles at the Lower Lateral Membrane of Polarized MDCK Cells

Li¹,

Hao

Cao³

et al. 2007

MBoC

View full text Add to dashboard Cite

Transforming growth factor-␣ (TGF-␣) is the major autocrine EGF receptor ligand in vivo.In polarized epithelial cells, proTGF-␣ is synthesized and then delivered to the basolateral cell surface. We previously reported that Naked2 interacts with basolateral sorting determinants in the cytoplasmic tail of a Golgi-processed form of TGF-␣ and that TGF-␣ is not detected at the basolateral surface of Madin-Darby canine kidney (MDCK) cells expressing myristoylation-deficient (G2A) Naked2. By high-resolution microscopy, we now show that wild-type, but not G2A, Naked2-associated vesicles fuse at the plasma membrane. We further demonstrate that Naked2-associated vesicles are delivered to the lower lateral membrane of polarized MDCK cells independent of 1B adaptin. We identify a basolateral targeting segment within Naked2; residues 1-173 redirect NHERF-1 from the apical cytoplasm to the basolateral membrane, and internal deletion of residues 37-104 results in apical mislocalization of Naked2 and TGF-␣. Short hairpin RNA knockdown of Naked2 leads to a dramatic reduction in the 16-kDa cell surface isoform of TGF-␣ and increased cytosolic TGF-␣ immunoreactivity. We propose that Naked2 acts as a cargo recognition and targeting (CaRT) protein to ensure proper delivery, tethering, and fusion of TGF-␣-containing vesicles to a distinct region at the basolateral surface of polarized epithelial cells. INTRODUCTION All seven mammalian EGF receptor (EGFR) ligands (EGF, TGF-␣ [TGF␣], amphiregulin, heparin-binding EGF-like growth factor, betacellulin, epiregulin and epigen) are type 1 transmembrane proteins that are produced by many epithelial cell types (Harris et al., 2003). The fidelity of trafficking of these endogenous EGFR ligands to the proper cell surface in normal polarized epithelial cells is highly relevant since the EGFR is restricted to the basolateral membrane. TGF␣ is delivered preferentially to the basolateral cell surface of polarized epithelial cells where it is rapidly cleaved by TNF␣converting enzyme/a disintegrin and metalloprotease (TACE/ADAM-17;Dempsey and Coffey, 1994;Sunnarborg et al., 2002). Soluble TGF␣ is then avidly captured by basolateral EGFRs (Dempsey and Coffey, 1994). The rapid cleavage and avid capture of this ligand suggest that cell surface delivery may be a critical, and possibly rate-limiting, step in the posttranslational regulation of endogenous TGF␣ activity.Basolateral sorting information usually resides in the cytoplasmic tail of basolaterally targeted cargo. TGF␣'s cytoplasmic tail, the most highly conserved portion of the molecule across species, contains domains that affect its trafficking through the secretory pathway. The C-terminus contains a type 1 PDZ recognition domain (ETVV). The PDZ-containing proteins syntenin (Fernandez-Larrea et al., 1999), GRASP55 (Kuo et al., 2000), and membrane-associated guanylate kinase inverted (MAGI)-2 and -3 (Franklin et al., 2005) bind this motif early in the secretory pathway. This domain contributes to the efficiency, but not the fidelity, of trafficki...

show abstract

Analysis of Membrane Traffic in Polarized Epithelial Cells

et al. 2001

Self Cite

View full text Add to dashboard Cite

Spatial asymmetry is fundamental to the structure and function of most eukaryotic cells. A basic aspect of this polarity is that the cell's plasma membrane is divided into discrete domains. The best studied and simplest example of this occurs in epithelial cells, which line exposed body surfaces. Epithelial cells use two pathways to send proteins to the cell surface. Newly made proteins can travel directly from the trans‐Golgi network (TGN) to either the apical or basolateral surface. Alternatively, proteins can be sent to the basolateral surface and then endocytosed and transcytosed to the apical surface. Epithelial cells grown on porous filters adopt a typical polarized morphology; transfected epithelial cells can be used to biosynthetically characterize the trafficking patterns of a given protein. These cells can also be used to study delivery to a particular surface and to localize the protein by immunofluorescence.

show abstract

Exocyst Is Involved in Cystogenesis and Tubulogenesis and Acts by Modulating Synthesis and Delivery of Basolateral Plasma Membrane and Secretory Proteins

Cited by 146 publications

References 91 publications

Intracellular signaling via ERK/MAPK completes the pathway for tubulogenic fibronectin in MDCK cells

Intracellular signaling via ERK/MAPK completes the pathway for tubulogenic fibronectin in MDCK cells

Naked2 Acts as a Cargo Recognition and Targeting Protein to Ensure Proper Delivery and Fusion of TGF-α–containing Exocytic Vesicles at the Lower Lateral Membrane of Polarized MDCK Cells

Analysis of Membrane Traffic in Polarized Epithelial Cells

Contact Info

Product

Resources

About