Two dileucine motifs mediate late endosomal/lysosomal targeting of transmembrane protein 192 (TMEM192) and a C-terminal cysteine residue is responsible for disulfide bond formation in TMEM192 homodimers

Jörg Behnke; Eeva-Liisa Eskelinen; Paul Saftig; Bernd Schröder

doi:10.1042/bj20101396

Two dileucine motifs mediate late endosomal/lysosomal targeting of transmembrane protein 192 (TMEM192) and a C-terminal cysteine residue is responsible for disulfide bond formation in TMEM192 homodimers

Biochemical Journal ◽

10.1042/bj20101396 ◽

2011 ◽

Vol 434 (2) ◽

pp. 219-231 ◽

Cited By ~ 15

Author(s):

Jörg Behnke ◽

Eeva-Liisa Eskelinen ◽

Paul Saftig ◽

Bernd Schröder

Keyword(s):

Disulfide Bond ◽

Disulfide Bonds ◽

Transmembrane Protein ◽

Bond Formation ◽

Immunogold Labelling ◽

Disulfide Bridge ◽

Cysteine Residue ◽

Disulfide Bond Formation ◽

Transmembrane Segments ◽

Late Endosomes

TMEM192 (transmembrane protein 192) is a novel constituent of late endosomal/lysosomal membranes with four potential transmembrane segments and an unknown function that was initially discovered by organellar proteomics. Subsequently, localization in late endosomes/lysosomes has been confirmed for overexpressed and endogenous TMEM192, and homodimers of TMEM192 linked by disulfide bonds have been reported. In the present study the molecular determinants of TMEM192 mediating its transport to late endosomes/lysosomes were analysed by using CD4 chimaeric constructs and mutagenesis of potential targeting motifs in TMEM192. Two directly adjacent N-terminally located dileucine motifs of the DXXLL-type were found to be critical for transport of TMEM192 to late endosomes/lysosomes. Whereas disruption of both dileucine motifs resulted in mistargeting of TMEM192 to the plasma membrane, each of the two motifs was sufficient to ensure correct targeting of TMEM192. In order to study disulfide bond formation, mutagenesis of cysteine residues was performed. Mutation of Cys266 abolished disulfide bridge formation between TMEM192 molecules, indicating that TMEM192 dimers are linked by a disulfide bridge between their C-terminal tails. According to the predicted topology, Cys266 would be localized in the reductive milieu of the cytosol where disulfide bridges are generally uncommon. Using immunogold labelling and proteinase protection assays, the localization of the N- and C-termini of TMEM192 on the cytosolic side of the late endosomal/lysosomal membrane was experimentally confirmed. These findings may imply close proximity of the C-termini in TMEM192 dimers and a possible involvement of this part of the protein in dimer assembly.

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Disulfide Bond Formation at the C Termini of Vaccinia Virus A26 and A27 Proteins Does Not Require Viral Redox Enzymes and Suppresses Glycosaminoglycan-Mediated Cell Fusion

Journal of Virology ◽

10.1128/jvi.02295-08 ◽

2009 ◽

Vol 83 (13) ◽

pp. 6464-6476 ◽

Cited By ~ 18

Author(s):

Yao-Cheng Ching ◽

Che-Sheng Chung ◽

Cheng-Yen Huang ◽

Yu Hsia ◽

Yin-Liang Tang ◽

...

Keyword(s):

Vaccinia Virus ◽

Cell Fusion ◽

Disulfide Bond ◽

Protein Complex ◽

Disulfide Bonds ◽

Bond Formation ◽

In Vitro Mutagenesis ◽

Disulfide Bond Formation ◽

Infected Cells

ABSTRACT Vaccinia virus A26 protein is an envelope protein of the intracellular mature virus (IMV) of vaccinia virus. A mutant A26 protein with a truncation of the 74 C-terminal amino acids was expressed in infected cells but failed to be incorporated into IMV (W. L. Chiu, C. L. Lin, M. H. Yang, D. L. Tzou, and W. Chang, J. Virol 81:2149-2157, 2007). Here, we demonstrate that A27 protein formed a protein complex with the full-length form but not with the truncated form of A26 protein in infected cells as well as in IMV. The formation of the A26-A27 protein complex occurred prior to virion assembly and did not require another A27-binding protein, A17 protein, in the infected cells. A26 protein contains six cysteine residues, and in vitro mutagenesis showed that Cys441 and Cys442 mediated intermolecular disulfide bonds with Cys71 and Cys72 of viral A27 protein, whereas Cys43 and Cys342 mediated intramolecular disulfide bonds. A26 and A27 proteins formed disulfide-linked complexes in transfected 293T cells, showing that the intermolecular disulfide bond formation did not depend on viral redox pathways. Finally, using cell fusion from within and fusion from without, we demonstrate that cell surface glycosaminoglycan is important for virus-cell fusion and that A26 protein, by forming complexes with A27 protein, partially suppresses fusion.

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A novelDFNA9mutation in the vWFA2 domain ofCOCHalters a conserved cysteine residue and intrachain disulfide bond formation resulting in progressive hearing loss and site-specific vestibular and central oculomotor dysfunction

American Journal of Medical Genetics Part A ◽

10.1002/ajmg.a.30980 ◽

2005 ◽

Vol 139A (2) ◽

pp. 86-95 ◽

Cited By ~ 44

Author(s):

Valerie A. Street ◽

Jeremy C. Kallman ◽

Nahid G. Robertson ◽

Sharon F. Kuo ◽

Cynthia C. Morton ◽

...

Keyword(s):

Hearing Loss ◽

Disulfide Bond ◽

Bond Formation ◽

Cysteine Residue ◽

Disulfide Bond Formation ◽

Progressive Hearing Loss ◽

Site Specific ◽

Intrachain Disulfide Bond

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Disulfide formation in plant storage vacuoles permits assembly of a multimeric lectin

Biochemical Journal ◽

10.1042/bj20091878 ◽

2010 ◽

Vol 427 (3) ◽

pp. 513-521 ◽

Cited By ~ 7

Author(s):

Richard S. Marshall ◽

Lorenzo Frigerio ◽

Lynne M. Roberts

Keyword(s):

Disulfide Bond ◽

Disulfide Bonds ◽

Castor Oil ◽

Ricinus Communis ◽

Bond Formation ◽

Disulfide Bond Formation ◽

Endosperm Tissue ◽

Oil Seed ◽

Protein Storage Vacuole ◽

Protein Disulfide

The ER (endoplasmic reticulum) has long been considered the plant cell compartment within which protein disulfide bond formation occurs. Members of the ER-located PDI (protein disulfide isomerase) family are responsible for oxidizing, reducing and isomerizing disulfide bonds, as well as functioning as chaperones to newly synthesized proteins. In the present study we demonstrate that an abundant 7S lectin of the castor oil seed protein storage vacuole, RCA (Ricinus communis agglutinin 1), is folded in the ER as disulfide bonded A–B dimers in both vegetative cells of tobacco leaf and in castor oil seed endosperm, but that these assemble into (A–B)2 disulfide-bonded tetramers only after Golgi-mediated delivery to the storage vacuoles in the producing endosperm tissue. These observations reveal an alternative and novel site conducive for disulfide bond formation in plant cells.

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Intracellular catalysis of disulfide bond formation by the human sulfhydryl oxidase, QSOX1

Biochemical Journal ◽

10.1042/bj20061510 ◽

2007 ◽

Vol 404 (3) ◽

pp. 403-411 ◽

Cited By ~ 63

Author(s):

Seema Chakravarthi ◽

Catherine E. Jessop ◽

Martin Willer ◽

Colin J. Stirling ◽

Neil J. Bulleid

Keyword(s):

Disulfide Bond ◽

Mammalian Cells ◽

Transmembrane Protein ◽

Bond Formation ◽

Secretory Protein ◽

Lung Fibroblasts ◽

Carboxypeptidase Y ◽

Disulfide Bond Formation ◽

Endometrial Cells

The discovery that the flavoprotein oxidase, Erv2p, provides oxidizing potential for disulfide bond formation in yeast, has led to investigations into the roles of the mammalian homologues of this protein. Mammalian homologues of Erv2p include QSOX (sulfhydryl oxidases) from human lung fibroblasts, guinea-pig endometrial cells and rat seminal vesicles. In the present study we show that, when expressed in mammalian cells, the longer version of human QSOX1 protein (hQSOX1a) is a transmembrane protein localized primarily to the Golgi apparatus. We also present the first evidence showing that hQSOX1a can act in vivo as an oxidase. Overexpression of hQSOX1a suppresses the lethality of a complete deletion of ERO1 (endoplasmic reticulum oxidase 1) in yeast and restores disulfide bond formation, as assayed by the folding of the secretory protein carboxypeptidase Y.

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Synthesis of bicyclic organo-peptide hybrids via oxime/intein-mediated macrocyclization followed by disulfide bond formation

Organic & Biomolecular Chemistry ◽

10.1039/c3ob42222d ◽

2014 ◽

Vol 12 (7) ◽

pp. 1135-1142 ◽

Cited By ~ 15

Author(s):

Jessica M. Smith ◽

Nicholas C. Hill ◽

Peter J. Krasniak ◽

Rudi Fasan

Keyword(s):

Disulfide Bond ◽

Bond Formation ◽

Disulfide Bridge ◽

Disulfide Bond Formation ◽

New Strategy ◽

Recombinant Polypeptides

A new strategy is described to convert recombinant polypeptides into bicyclic organo-peptide hybrids constrained by an intramolecular disulfide bridge.

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Cardiac peroxiredoxins undergo complex modifications during cardiac oxidant stress

AJP Heart and Circulatory Physiology ◽

10.1152/ajpheart.00017.2008 ◽

2008 ◽

Vol 295 (1) ◽

pp. H425-H433 ◽

Cited By ~ 37

Author(s):

Ewald Schröder ◽

Jonathan P. Brennan ◽

Philip Eaton

Keyword(s):

Hydrogen Peroxide ◽

Disulfide Bond ◽

Disulfide Bonds ◽

Structural Changes ◽

Oxidant Stress ◽

Bond Formation ◽

Redox Signaling ◽

Size Exclusion ◽

Disulfide Bond Formation ◽

Dimeric Unit

Peroxiredoxins (Prdxs), a family of antioxidant and redox-signaling proteins, are plentiful within the heart; however, their cardiac functions are poorly understood. These studies were designed to characterize the complex changes in Prdxs induced by oxidant stress in rat myocardium. Hydrogen peroxide, a Prdx substrate, was used as the model oxidant pertinent to redox signaling during health and to injury at higher concentrations. Rat hearts were aerobically perfused with a broad concentration range of hydrogen peroxide by the Langendorff method, homogenized, and analyzed by immunoblotting. Heart extracts were also analyzed by size-exclusion chromatography under nondenaturing conditions. Hydrogen peroxide-induced changes in disulfide bond formation, nonreversible oxidation of cysteine (hyperoxidation), and subcellular localization were determined. Hydrogen peroxide induced an array of changes in the myocardium, including formation of disulfide bonds that were intermolecular for Prdx1, Prdx2, and Prdx3 but intramolecular within Prdx5. For Prdx1, Prdx2, and Prdx5, disulfide bond formation can be approximated to an EC50 of 10–100, 1–10, and 100–1,000 μM peroxide, respectively. Hydrogen peroxide induced hyperoxidation, not just within monomeric Prdx (by SDS-PAGE), but also within Prdx disulfide dimers, and reflects a flexibility within the dimeric unit. Prdx oxidation was also associated with movement from the cytosolic to the membrane and myofilament-enriched fractions. In summary, Prdxs undergo a complex series of redox-dependent structural changes in the heart in response to oxidant challenge with its substrate hydrogen peroxide.

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Functional Domain of Bovine Milk Lactoferrin Which Inhibits the Adherence of Streptococcus mutans Cells to a Salivary Film

Infection and Immunity ◽

10.1128/iai.70.9.5279-5282.2002 ◽

2002 ◽

Vol 70 (9) ◽

pp. 5279-5282 ◽

Cited By ~ 26

Author(s):

Takahiko Oho ◽

Morihide Mitoma ◽

Toshihiko Koga

Keyword(s):

Streptococcus Mutans ◽

Disulfide Bond ◽

Bond Formation ◽

Bovine Milk ◽

Cysteine Residue ◽

Bovine Lactoferrin ◽

Functional Domain ◽

Disulfide Bond Formation ◽

Serine Residue

ABSTRACT The bovine lactoferrin molecule and relatively long lactoferrin fragments containing residues 473 to 538 strongly inhibited adherence of Streptococcus mutans to saliva-coated hydroxyapatite beads. Each cysteine residue in Lf411 (residues 473 to 538) was replaced by a serine residue, and the mutants Lf411-C481S and Lf411-C532S strongly inhibited S. mutans adherence. These results suggest that the functional domain of lactoferrin that binds to a salivary film lies in residues 473 to 538 and that the region might be concealed by disulfide bond formation between Cys481 and Cys532 in the Lf411 fragment.

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Applications of catalyzed cytoplasmic disulfide bond formation

Biochemical Society Transactions ◽

10.1042/bst20190088 ◽

2019 ◽

Vol 47 (5) ◽

pp. 1223-1231 ◽

Cited By ~ 1

Author(s):

Mirva J. Saaranen ◽

Lloyd W. Ruddock

Keyword(s):

Disulfide Bond ◽

Disulfide Bonds ◽

Molecular Mechanisms ◽

Bond Formation ◽

Disulfide Bond Formation ◽

Post Translational Modification ◽

Natural Systems ◽

Cell Factories ◽

Engineered Systems ◽

Disulfide Isomerization

Abstract Disulfide bond formation is an essential post-translational modification required for many proteins to attain their native, functional structure. The formation of disulfide bonds, otherwise known as oxidative protein folding, occurs in the endoplasmic reticulum and mitochondrial inter-membrane space in eukaryotes and the periplasm of prokaryotes. While there are differences in the molecular mechanisms of oxidative folding in different compartments, it can essentially be broken down into two steps, disulfide formation and disulfide isomerization. For both steps, catalysts exist in all compartments where native disulfide bond formation occurs. Due to the importance of disulfide bonds for a plethora of proteins, considerable effort has been made to generate cell factories which can make them more efficiently and cheaper. Recently synthetic biology has been used to transfer catalysts of native disulfide bond formation into the cytoplasm of prokaryotes such as Escherichia coli. While these engineered systems cannot yet rival natural systems in the range and complexity of disulfide-bonded proteins that can be made, a growing range of proteins have been made successfully and yields of homogenously folded eukaryotic proteins exceeding g/l yields have been obtained. This review will briefly give an overview of such systems, the uses reported to date and areas of future potential development, including combining with engineered systems for cytoplasmic glycosylation.

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ATP Is Required for Correct Folding and Disulfide Bond Formation of Rotavirus VP7

Journal of Virology ◽

10.1128/jvi.74.17.8048-8052.2000 ◽

2000 ◽

Vol 74 (17) ◽

pp. 8048-8052 ◽

Cited By ~ 18

Author(s):

Ali Mirazimi ◽

Lennart Svensson

Keyword(s):

Disulfide Bond ◽

Disulfide Bonds ◽

Semliki Forest Virus ◽

Energy State ◽

Energy Requirement ◽

Expression System ◽

Bond Formation ◽

Minimum Energy ◽

Metabolic Energy ◽

Disulfide Bond Formation

ABSTRACT Rotavirus is one of very few viruses that utilize the endoplasmic reticulum (ER) for assembly, and therefore it has been used as an attractive model to study ER-associated protein folding. In this study, we have examined the requirements for metabolic energy (ATP) for correct folding of the luminal and ER-associated VP7 of rotavirus. We found that VP7 rapidly misfolds in an energy-depleted milieu and is not degraded within 60 min. We also found that VP7 attained a stable minimum-energy state soon after translation in the ER. Most surprisingly, energy-misfolded VP7 could be recovered and establish correct disulfide bonds and antigenicity following a shift to an ATP-rich milieu. Using a Semliki Forest virus expression system, we observed that VP7 requires ATP and cellular, but not viral, factors for correct disulfide bond formation. Our results show for the first time that the disulfide bond formation of rotavirus VP7 is an ATP-dependent process. It has previously been shown that chaperones hydrolyze ATP during interaction with newly synthesized polypeptides and prevent nonproductive intra- and intermolecular interactions. The most reasonable explanation for the energy requirement of VP7 is thus a close interaction during folding with an ATP-dependent chaperone, such as BiP (Grp78), and possibly with protein disulfide isomerase. Taken together, our observations provide new information about folding of ER-associated proteins in general and rotavirus VP7 in particular.

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Per Os Infectivity Factor 5 Identified as a Substrate of P33 in the Baculoviral Disulfide Bond Formation Pathway

Journal of Virology ◽

10.1128/jvi.00615-20 ◽

2020 ◽

Vol 94 (15) ◽

Author(s):

Huanyu Zhang ◽

Wenhua Kuang ◽

Cheng Chen ◽

Yu Shang ◽

Xiaoyan Ma ◽

...

Keyword(s):

Disulfide Bond ◽

Disulfide Bonds ◽

Bond Formation ◽

Oral Infection ◽

Progeny Virus ◽

Disulfide Bond Formation ◽

Sulfhydryl Oxidase ◽

Dna Viruses ◽

Formation Pathway

ABSTRACT Disulfide bonds are critical for the structure and function of many proteins. Some large DNA viruses encode their own sulfhydryl oxidase for disulfide bond formation. Previous studies have demonstrated that the baculovirus-encoded sulfhydryl oxidase P33 is necessary for progeny virus production, and its enzymatic activity is important for morphogenesis and oral infectivity of baculoviruses. However, the downstream substrates of P33 in the putative redox pathway of baculoviruses are unknown. In this study, we showed that PIF5, one of the per os infectivity factors (PIFs), contained intramolecular disulfide bonds and that the disulfide bond formation was interrupted in the absence of P33. In vivo pulldown and colocalization analyses revealed that PIF5 and P33 interacted with each other during virus infection. Further, in vitro assays validated that the reduced PIF5 proteins could be oxidized by P33. To understand the contribution of disulfide bonds to the function of PIF5, several cysteine-to-serine mutants were constructed, which all interfered with the disulfide bond formation of PIF5 to different extents. All the mutants lost their oral infectivity but had no impact on infectious budding virus (BV) production or virus morphogenesis. Taken together, our results indicated PIF5 as the first identified substrate of P33. Further, the disulfide bonds in PIF5 play an essential role in its function in oral infection. IMPORTANCE Similar to some large DNA viruses that encode their own disulfide bond pathway, baculovirus encodes a viral sulfhydryl oxidase, P33. Enzyme activity of P33 is related to infectious BV production, occlusion-derived virus (ODV) envelopment, occlusion body morphogenesis, and oral infectivity, suggesting that P33 is involved in disulfide bond formation of multiple proteins. A complete disulfide bond formation pathway normally contains a sulfhydryl oxidase, a disulﬁde-donating enzyme, and one or more substrates. In baculovirus, apart from P33, other components of the putative pathway remain unknown. In this study, we identified PIF5 as the first substrate of P33, which is fundamental for revealing the complete disulfide bond formation pathway in baculovirus. PIF5 is essential for oral infection and is absent from the PIF complex. Our study demonstrated that native disulfide bonds in PIF5 are required for oral infection, which will help us to reveal its mode of action.

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