Rescue of Munc18-1 and -2 Double Knockdown Reveals the Essential Functions of Interaction between Munc18 and Closed Syntaxin in PC12 Cells

Han, Liping; Jiang, Tiandan; Han, Gayoung A.; Malintan, Nancy T.; Xie, Lin; Wang, Li; Tse, Frederick W.; Gaisano, Herbert Y.; Collins, Brett M.; Meunier, Frédéric A.; Sugita, Shuzo

doi:10.1091/mbc.e09-08-0712

Cited by 73 publications

(139 citation statements)

References 61 publications

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“…We previously found that Munc18-1/2 DKD causes not only a strong reduction in syntaxin-1 level but also perturbation of its plasmalemmal localization in PC12 cells (15,16). We therefore examined whether the subcellular localization of syntaxin-11 can be significantly altered by Munc18-1/2 DKD in RBL-2H3 cells ( Fig.…”

Section: Resultsmentioning

confidence: 98%

“…The lack of rescue by the hydrophobic pocket mutants in Munc18-2 is surprising, as we previously found that the expressions of Munc18-1 with the identical mutations showed 70-80% of the rescue ability compared with the wild type, using Munc18-1 KD and Munc18-1/2 DKD PC12 cells (15,31). Furthermore, the same (F115E) and a similar (L130K) mutant have shown a complete rescue ability in autaptic neurotransmission of Munc18-1-deficient neurons (32).…”

Section: Munc18-1 and Munc18-2 Can Effectively Support Mast Cell Degrmentioning

confidence: 88%

“…The Munc18 family of proteins has been revealed to play multiple functions, which include both chaperoning cognate syntaxins (14)(15)(16)(17)(18)(19) and priming/stimulating membrane fusion through interaction with the SNARE complex (20-23) (reviewed in ref. 24).…”

mentioning

confidence: 99%

“…The chaperoning function of Munc18 contributes to stabilizing the expression level of cognate syntaxins and, in some cases, trafficking them to the appropriate intracellular compartments. For instance, in Munc18-1-deficient neurons, the syntaxin-1 level is reduced by 50-75% (3), whereas in Munc18-1 single-knockdown (KD) and Munc18-1/2 double-knockdown (DKD) pheochromocytoma (PC) 12 cells, not only the reduction of syntaxin-1 expression level but also its localization at the plasma membrane are severely perturbed (14,15). In some patients with FHL5 whose functional Munc18-2 protein is absent, a strong reduction in syntaxin-11 level was found in their immune cells (11,12).…”

mentioning

confidence: 99%

“…In contrast, the Munc18-1 hydrophobic pocket has been suggested to play limited or dispensable roles in exocytosis. For example, in the rescue experiments of Munc18-1 single-KD and Munc18-1/2 DKD PC12 cells as well as Munc18-1 knockout neurons, various mutants (F115E, E132A, F115E/ E132A, and L130K) in the hydrophobic pocket region of Munc18-1 have exhibited either very mild or no impairment in their ability to rescue exocytosis in comparison with the wild type (15,31,32), leaving the function of the hydrophobic pocket region of Munc18 unclear.…”

mentioning

confidence: 99%

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Crucial role of the hydrophobic pocket region of Munc18 protein in mast cell degranulation

Bin

Jung

Piggott

et al. 2013

Proc. Natl. Acad. Sci. U.S.A.

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The function of the Munc18-1 protein hydrophobic pocket, which interacts with the syntaxin-1 N-terminal peptide, has been highly controversial in neurosecretion. Recent analysis of patients with familial hemophagocytic lymphohistiocytosis type 5 has identified the E132A mutation in the hydrophobic pocket of Munc18-2, prompting us to examine the role of this region in the context of immune cell secretion. Double knockdown of Munc18-1 and Munc18-2 in RBL-2H3 mast cells eliminates both IgE-dependent and ionomycin-induced degranulation and causes a significant reduction in syntaxin-11 without altering expressions of the other syntaxin isoforms examined. These phenotypes were effectively rescued on reexpression of wild-type Munc18-1 or Munc18-2 but not the mutants (F115E, E132A, and F115E/E132A) in the hydrophobic pocket of Munc18. In addition, these mutants show that they are unable to directly interact with syntaxin-11, as tested through protein interaction experiments. Our results demonstrate the crucial roles of the hydrophobic pocket of Munc18 in mast cell degranulation, which include the regulation of syntaxin-11. We also suggest that the functional importance of this region is significantly different between neuronal and immune cell exocytosis.membrane fusion | FHL5

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Section: Resultsmentioning

confidence: 98%

Section: Munc18-1 and Munc18-2 Can Effectively Support Mast Cell Degrmentioning

confidence: 88%

mentioning

confidence: 99%

mentioning

confidence: 99%

mentioning

confidence: 99%

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Crucial role of the hydrophobic pocket region of Munc18 protein in mast cell degranulation

Bin

Jung

Piggott

et al. 2013

Proc. Natl. Acad. Sci. U.S.A.

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Survey of the year 2009: applications of isothermal titration calorimetry

Falconer

Collins

2010

J. Mol. Recognit.

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Isothermal titration calorimetry (ITC) is now an established and invaluable method for determining the thermodynamic constants, association constant and stoichiometry of molecular interactions in aqueous solutions. The technique has become widely used by biochemists to study protein interaction with other proteins, small molecules, metal ions, lipids, nucleic acids and carbohydrates; and nucleic acid interaction with small molecules. The drug discovery industry has utilized this approach to measure protein (or nucleic acid) interaction with drug candidates. ITC has been used to screen candidates, guide the design of potential drugs and validate the modelling used in structure-based drug design. Emerging disciplines including nanotechnology and drug delivery could benefit greatly from ITC in enhancing their understanding and control of nano-particle assembly, and drug binding and controlled release.

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Protein structure and phenotypic analysis of pathogenic and population missense variants inSTXBP1

Suri

Evers

Laskowski

et al. 2017

Mol Genet Genomic Med

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BackgroundSyntaxin‐binding protein 1, encoded by STXBP1, is highly expressed in the brain and involved in fusing synaptic vesicles with the plasma membrane. Studies have shown that pathogenic loss‐of‐function variants in this gene result in various types of epilepsies, mostly beginning early in life. We were interested to model pathogenic missense variants on the protein structure to investigate the mechanism of pathogenicity and genotype–phenotype correlations.MethodsWe report 11 patients with pathogenic de novo mutations in STXBP1 identified in the first 4293 trios of the Deciphering Developmental Disorder (DDD) study, including six missense variants. We analyzed the structural locations of the pathogenic missense variants from this study and the literature, as well as population missense variants extracted from Exome Aggregation Consortium (ExAC).ResultsPathogenic variants are significantly more likely to occur at highly conserved locations than population variants, and be buried inside the protein domain. Pathogenic mutations are also more likely to destabilize the domain structure compared with population variants, increasing the proportion of (partially) unfolded domains that are prone to aggregation or degradation. We were unable to detect any genotype–phenotype correlation, but unlike previously reported cases, most of the DDD patients with STXBP1 pathogenic variants did not present with very early‐onset or severe epilepsy and encephalopathy, though all have developmental delay with intellectual disability and most display behavioral problems and suffered seizures in later childhood.ConclusionVariants across STXBP1 that cause loss of function can result in severe intellectual disability with or without seizures, consistent with a haploinsufficiency mechanism. Pathogenic missense mutations act through destabilization of the protein domain, making it prone to aggregation or degradation. The presence or absence of early seizures may reflect ascertainment bias in the literature as well as the broad recruitment strategy of the DDD study.

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Rescue of Munc18-1 and -2 Double Knockdown Reveals the Essential Functions of Interaction between Munc18 and Closed Syntaxin in PC12 Cells

Cited by 73 publications

References 61 publications

Crucial role of the hydrophobic pocket region of Munc18 protein in mast cell degranulation

Crucial role of the hydrophobic pocket region of Munc18 protein in mast cell degranulation

Survey of the year 2009: applications of isothermal titration calorimetry

Protein structure and phenotypic analysis of pathogenic and population missense variants inSTXBP1

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