N-terminal Domains Elicit Formation of Functional Pmel17 Amyloid Fibrils

Watt, Brenda; Niel, Guillaume van; Fowler, Douglas M.; Hurbain, Ilse; Luk, Kelvin C.; Stayrook, Steven E.; Lemmon, Mark A.; Raposo, Graça; Shorter, James; Kelly, Jeffery W.; Marks, Michael S.

doi:10.1074/jbc.m109.047449

Cited by 102 publications

(163 citation statements)

References 57 publications

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“…S4B). When they have been released from the membrane in control cells, Mα fragments assemble into Triton X-100 (TX)-insoluble fibrils (12) and undergo further proteolytic processing to smaller fragments (detected by antibodies HMB45 and I51) (16,26,27) (Fig. S1A).…”

Section: Bace2 Releases Pmel Luminal Domain To Generate Amyloidogenicmentioning

confidence: 99%

“…S1A). They include (i) cleavage of the full-length transmembrane form of PMEL by a proprotein convertase (PC) into an amyloidogenic luminal Mα fragment and a disulfide-linked transmembrane domain-containing Mβ fragment (12), (ii) further cleavage of Mβ by an "endosomal" sheddase to release Mα linked to Mβ luminal domain (i.e., Mβ-N) from the transmembrane C-terminal fragment (CTF) and to allow Mα oligomerization to form amyloid fibrils (13,14), (iii) further processing of Mα by unknown proteases into smaller fragments found in mature fibrils and fibrillar sheets (15,16), and (iv) intramembrane proteolysis of the CTF by the γ-secretase complex (13,14). The analogy between the processing of PMEL and APP led us to investigate the role of BACE secretases in PMEL processing and functional amyloid formation.…”

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confidence: 99%

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BACE2 processes PMEL to form the melanosome amyloid matrix in pigment cells

Rochin

Hurbain

Serneels

et al. 2013

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

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143

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Amyloids are often associated with pathologic processes such as in Alzheimer's disease (AD), but can also underlie physiological processes such as pigmentation. Formation of pathological and functional amyloidogenic substrates can require precursor processing by proteases, as exemplified by the generation of Aβ peptide from amyloid precursor protein (APP) by beta-site APP cleaving enzyme (BACE)1 and γ-secretase. Proteolytic processing of the pigment cell-specific Melanocyte Protein (PMEL) is also required to form functional amyloid fibrils during melanogenesis, but the enzymes involved are incompletely characterized. Here we show that the BACE1 homologue BACE2 processes PMEL to generate functional amyloids. BACE2 is highly expressed in pigment cells and Bace2 −/− but not Bace1 −/− mice display coat color defects, implying a specific role for BACE2 during melanogenesis. By using biochemical and morphological analyses, combined with RNA silencing, pharmacologic inhibition, and BACE2 overexpression in a human melanocytic cell line, we show that BACE2 cleaves the integral membrane form of PMEL within the juxtamembrane domain, releasing the PMEL luminal domain into endosomal precursors for the formation of amyloid fibrils and downstream melanosome morphogenesis. These studies identify an amyloidogenic substrate of BACE2, reveal an important physiological role for BACE2 in pigmentation, and highlight analogies in the generation of PMEL-derived functional amyloids and APPderived pathological amyloids.

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Section: Bace2 Releases Pmel Luminal Domain To Generate Amyloidogenicmentioning

confidence: 99%

mentioning

confidence: 99%

BACE2 processes PMEL to form the melanosome amyloid matrix in pigment cells

Rochin

Hurbain

Serneels

et al. 2013

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

Self Cite

143

166

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“…Though there is no current consensus as to which polypeptide domain solely or partly constitutes the Pmel17 amyloid core, recent results showed that both isolated luminal regions, RPT, residues 315-444 ( Fig. 1) (24) and the polycystic kidney disease-1 like domain, residues 201-314 (25) are sufficient for amyloid formation in vitro. While both domains are important for fibril formation in vivo (26), we choose RPTas a model system to study aggregation kinetics because prior observation revealed that RPT fibril stability is particularly pH sensitive (24).…”

mentioning

confidence: 99%

Effects of pH on aggregation kinetics of the repeat domain of a functional amyloid, Pmel17

Pfefferkorn

McGlinchey²,

Lee³

2010

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

114

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Pmel17 is a functional amyloidogenic protein whose fibrils act as scaffolds for pigment deposition in human skin and eyes. We have used the repeat domain (RPT, residues 315-444), an essential luminal polypeptide region of Pmel17, as a model system to study conformational changes from soluble unstructured monomers to β-sheet-containing fibrils. Specifically, we report on the effects of solution pH (4 → 7) mimicking pH conditions of melanosomes, acidic organelles where Pmel17 fibrils are formed. Local, secondary, and fibril structure were monitored via intrinsic Trp fluorescence, circular dichroism spectroscopy, and transmission electron microscopy, respectively. We find that W423 is a highly sensitive probe of amyloid assembly with spectral features reflecting local conformational and fibril morphological changes. A critical pH regime (5 AE 0.5) was identified for fibril formation suggesting the involvement of at least three carboxylic acids in the structural rearrangement necessary for aggregation. Moreover, we demonstrate that RPT fibril morphology can be transformed directly by changing solution pH. Based on these results, we propose that intramelanosomal pH regulates Pmel17 amyloid formation and its subsequent dissolution in vivo.fibril | fluorescence | melanosome | tryptophan | melanin

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“…The conversion of full-length wild type and mutant Cdk5-phosphorylated PrPs occurs at physiological pH and temperature and in non-denaturant conditions, similar to that observed for the human Pmel17 Ma fragment, which readily converts into amyloid and forms the core of melanosomes (41). The IKTA reaction indicates first order kinetics for the Cdk5-mediated conversion of wild type and mutant full-length PrPs, similar to that obtained with other functional amyloid-forming proteins from fungi to mammals (41)(42)(43)(44)(45)(46)(47). Furthermore, the ThT-positive amyloid in PrP WT-V or Y145X M and the seeding properties of phosphorylated Q160X M were partially reversible upon dephosphorylation, similar to the reversibility of secretory granule peptide hormone amyloids as they convert to a monomeric ␣-helical form when released (45).…”

Section: Discussionmentioning

confidence: 71%

Cyclin-dependent Kinase 5 Phosphorylation of Familial Prion Protein Mutants Exacerbates Conversion into Amyloid Structure

Rouget

Sharma

LeBlanc

2015

Journal of Biological Chemistry

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Background: Conversion of prion protein occurs in familial prion diseases, but the exact mechanism is unknown. Results: Phosphorylation at the N-terminal serine 43 causes or exacerbates conversion of familial prion protein mutants. Conclusion:The N terminus and C terminus of prion protein both influence conversion into amyloid. Significance: The flexible N terminus of prion protein plays a role in amyloid conversion and could indicate a novel target to prevent prion conversion.

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N-terminal Domains Elicit Formation of Functional Pmel17 Amyloid Fibrils

Cited by 102 publications

References 57 publications

BACE2 processes PMEL to form the melanosome amyloid matrix in pigment cells

BACE2 processes PMEL to form the melanosome amyloid matrix in pigment cells

Effects of pH on aggregation kinetics of the repeat domain of a functional amyloid, Pmel17

Cyclin-dependent Kinase 5 Phosphorylation of Familial Prion Protein Mutants Exacerbates Conversion into Amyloid Structure

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