Identification of ERGIC-53 as an intracellular transport receptor of α1-antitrypsin

Secretory proteins are exported from the endoplasmic reticulum (ER) by bulk flow and/or receptor-mediated transport. Our understanding of this process is limited because of the low number of identified transport receptors and cognate cargo proteins. In mammalian cells, the lectin ER Golgi intermediate compartment 53-kD protein (ERGIC-53) represents the best characterized cargo receptor. It assists ER export of a subset of glycoproteins including coagulation factors V and VIII and cathepsin C and Z. Here, we report a novel screening strategy to identify protein interactions in the lumen of the secretory pathway using a yellow fluorescent protein–based protein fragment complementation assay. By screening a human liver complementary DNA library, we identify α1-antitrypsin (α1-AT) as previously unrecognized cargo of ERGIC-53 and show that cargo capture is carbohydrate- and conformation-dependent. ERGIC-53 knockdown and knockout cells display a specific secretion defect of α1-AT that is corrected by reintroducing ERGIC-53. The results reveal ERGIC-53 to be an intracellular transport receptor of α1-AT and provide direct evidence for active receptor-mediated ER export of a soluble secretory protein in higher eukaryotes.

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Visualization of protein interactions inside the secretory pathway

Biochemical Society Transactions ◽

10.1042/bst0350970 ◽

2007 ◽

Vol 35 (5) ◽

pp. 970-973 ◽

Cited By ~ 9

Author(s):

B. Nyfeler ◽

H.-P. Hauri

Keyword(s):

Endoplasmic Reticulum ◽

Protein Interactions ◽

Secretory Pathway ◽

Fluorescent Protein ◽

Yellow Fluorescent Protein ◽

Coagulation Factor ◽

Cdna Libraries ◽

Major Protein ◽

Protein Protein Interactions ◽

A Genome

The ER (endoplasmic reticulum) is a major protein folding and modification organelle. In its lumen, the ER processes a third of all newly synthesized proteins. To accomplish this task, numerous resident proteins capture the nascent and newly synthesized proteins. The underlying luminal protein–protein interactions, however, are inherently difficult to analyse, mainly due to their transient nature and the rather specialized environment of the ER. To overcome these limitations, we developed a PCA (protein fragment complementation assay) based on the citrine variant of YFP (yellow fluorescent protein). YFP PCA was successfully applied to visualize the protein interactions of the cargo transport receptor ERGIC-53 (endoplasmic reticulum–Golgi intermediate compartment protein of 53 kDa) with its luminal interaction partner MCFD2 (multiple coagulation factor deficiency protein 2) and its cargo proteins cathepsin Z and cathepsin C in a specific manner. With the prospect of screening cDNA libraries for novel protein–protein interactions, YFP PCA is a promising emerging technique for mapping protein interactions inside the secretory pathway in a genome-wide setting.

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Unfolded Protein Response Pathways in Bloodstream-Form Trypanosoma brucei?

Eukaryotic Cell ◽

10.1128/ec.00118-15 ◽

2015 ◽

Vol 14 (11) ◽

pp. 1094-1101 ◽

Cited By ~ 7

Author(s):

Calvin Tiengwe ◽

Abigail E. N. A. Brown ◽

James D. Bangs

Keyword(s):

Er Stress ◽

Unfolded Protein Response ◽

Trypanosoma Brucei ◽

Mammalian Cells ◽

Secretory Pathway ◽

Secretory Protein ◽

Secretory Proteins ◽

African Trypanosomes ◽

Unfolded Protein ◽

Protein Response

ABSTRACT The unfolded protein response (UPR) is a stress mechanism to cope with misfolded proteins in the early secretory pathway, the hallmark being transcriptional upregulation of endoplasmic reticulum (ER) molecular chaperones such as BiP and protein disulfide isomerase. Despite the lack of transcriptional regulation and the absence of the classical UPR machinery, African trypanosomes apparently respond to persistent ER stress by a UPR-like response, including upregulation of BiP, and a related spliced leader silencing (SLS) response whereby SL RNA transcription is shut down. Initially observed by knockdown of the secretory protein translocation machinery, both responses are also induced by chemical agents known to elicit UPR in mammalian cells (H. Goldshmidt, D. Matas, A. Kabi, A. Carmi, R. Hope, S. Michaeli, PLoS Pathog 6:e1000731, 2010, http://dx.doi.org/10.1371/journal.ppat.1000731 ). As these findings were generated primarily in procyclic-stage trypanosomes, we have investigated both responses in pathogenic bloodstream-stage parasites. RNA interference (RNAi) silencing of the core translocon subunit Trypanosoma brucei Sec61α (TbSec61α) failed to induce either response. Interestingly, cell growth halted within 16 h of silencing, but sufficient TbSec61α remained to allow full competence for translocation of nascent secretory proteins for up to 24 h, indicating that replication is finely coupled with the capacity to synthesize and transport secretory cargo. Tunicamycin and thapsigargin at concentrations compatible with short-term (4 h) and long-term (24 h) viability also failed to induce any of the indicators of UPR-like or SLS responses. Dithiothreitol (DTT) was lethal at all concentrations tested. These results indicate that UPR-like and SLS responses to persistent ER stress do not occur in bloodstream-stage trypanosomes.

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Enhanced brightness of bacterial luciferase by bioluminescence resonance energy transfer

Scientific Reports ◽

10.1038/s41598-021-94551-4 ◽

2021 ◽

Vol 11 (1) ◽

Author(s):

Tomomi Kaku ◽

Kazunori Sugiura ◽

Tetsuyuki Entani ◽

Kenji Osabe ◽

Takeharu Nagai

Keyword(s):

Energy Transfer ◽

Mammalian Cells ◽

Fluorescent Protein ◽

Color Change ◽

Yellow Fluorescent Protein ◽

Resonance Energy Transfer ◽

Resonance Energy ◽

Bioluminescence Resonance Energy Transfer ◽

Bacterial Luciferase ◽

Bacterial Bioluminescence

AbstractUsing the lux operon (luxCDABE) of bacterial bioluminescence system as an autonomous luminous reporter has been demonstrated in bacteria, plant and mammalian cells. However, applications of bacterial bioluminescence-based imaging have been limited because of its low brightness. Here, we engineered the bacterial luciferase (heterodimer of luxA and luxB) by fusion with Venus, a bright variant of yellow fluorescent protein, to induce bioluminescence resonance energy transfer (BRET). By using decanal as an externally added substrate, color change and ten-times enhancement of brightness was achieved in Escherichia coli when circularly permuted Venus was fused to the C-terminus of luxB. Expression of the Venus-fused luciferase in human embryonic kidney cell lines (HEK293T) or in Nicotiana benthamiana leaves together with the substrate biosynthesis-related genes (luxC, luxD and luxE) enhanced the autonomous bioluminescence. We believe the improved luciferase will forge the way towards the potential development of autobioluminescent reporter system allowing spatiotemporal imaging in live cells.

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Dynamic tracking and identification of tissue-specific secretory proteins in the circulation of live mice

10.21203/rs.3.rs-90987/v1 ◽

2020 ◽

Author(s):

Jae Myoung Suh ◽

Kwang-eun Kim ◽

Isaac Park ◽

Jeesoo Kim ◽

Myeong-Gyun Kang ◽

...

Keyword(s):

Blood Plasma ◽

Mouse Liver ◽

Secretory Pathway ◽

Secretory Protein ◽

Protein Labeling ◽

Secretory Proteins ◽

Tissue Specific ◽

Dynamic Tracking

Abstract Here we describe iSLET (in situ Secretory protein Labeling via ER-anchored TurboID) which labels secretory pathway proteins as they transit through the ER-lumen to enable dynamic tracking of tissue-specific secreted proteomes in vivo. We expressed iSLET in the mouse liver and demonstrated efficient in situ labeling of the liver-specific secreted proteome which could be tracked and identified within circulating blood plasma. iSLET is a versatile and powerful tool for studying spatiotemporal dynamics of secretory proteins, a valuable class of biomarkers and therapeutic targets.

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An antibody against secretogranin I (chromogranin B) is packaged into secretory granules.

The Journal of Cell Biology ◽

10.1083/jcb.109.1.17 ◽

1989 ◽

Vol 109 (1) ◽

pp. 17-34 ◽

Cited By ~ 73

Author(s):

P Rosa ◽

U Weiss ◽

R Pepperkok ◽

W Ansorge ◽

C Niehrs ◽

...

Keyword(s):

Secretory Pathway ◽

Secretory Granules ◽

Intracellular Localization ◽

Secretory Protein ◽

Secretory Proteins ◽

Chromogranin B ◽

Double Labeling ◽

Protein Protein Interaction ◽

And Function ◽

Secretogranin I

We have investigated the sorting and packaging of secretory proteins into secretory granules by an immunological approach. An mAb against secretogranin I (chromogranin B), a secretory protein costored with various peptide hormones and neuropeptides in secretory granules of many endocrine cells and neurons, was expressed by microinjection of its mRNA into the secretogranin I-producing cell line PC12. An mAb against the G protein of vesicular stomatitis virus--i.e., against an antigen not present in PC12 cells--was expressed as a control. The intracellular localization and the secretion of the antibodies was studied by double-labeling immunofluorescence using the conventional and the confocal microscope, as well as by pulse-chase experiments. The secretogranin I antibody, like the control antibody, was transported along the secretory pathway to the Golgi complex. However, in contrast to the control antibody, which was secreted via the constitutive pathway, the secretogranin I antibody formed an immunocomplex with secretogranin I, was packaged into secretory granules, and was released by regulated exocytosis. Our results show that a constitutive secretory protein, unaltered by genetic engineering, can be diverted to the regulated pathway of secretion by its protein-protein interaction with a regulated secretory protein. The data also provide the basis for immunologically studying the role of luminally exposed protein domains in the biogenesis and function of regulated secretory vesicles.

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Depletion of rafts in late endocytic membranes is controlled by NPC1-dependent recycling of cholesterol to the plasma membrane

Journal of Cell Science ◽

10.1242/jcs.114.10.1893 ◽

2001 ◽

Vol 114 (10) ◽

pp. 1893-1900 ◽

Cited By ~ 3

Author(s):

S. Lusa ◽

T.S. Blom ◽

E.L. Eskelinen ◽

E. Kuismanen ◽

J.E. Mansson ◽

...

Keyword(s):

Plasma Membrane ◽

Protein Interactions ◽

Mammalian Cells ◽

Intracellular Transport ◽

Ldl Cholesterol ◽

Normal Cells ◽

Recycling Endosomes ◽

Regulate Protein ◽

Niemann Pick ◽

Accumulation Characteristic

In mammalian cells, cholesterol is thought to associate with sphingolipids to form lateral membrane domains termed rafts. Increasing evidence suggests that rafts regulate protein interactions, for example, during signalling, intracellular transport and host-pathogen interactions. Rafts are present in cholesterol-sphingolipid-enriched membranes, including early and recycling endosomes, but whether rafts are found in late endocytic organelles has not been analyzed. In this study, we analyzed the association of cholesterol and late endosomal proteins with low-density detergent-resistant membranes (DRMs) in normal cells and in cells with lysosomal cholesterol-sphingolipid accumulation. In normal cells, the majority of [(3)H]cholesterol released from [(3)H]cholesterol ester-LDL associated with detergent-soluble membranes, was rapidly transported to the plasma membrane and became increasingly insoluble with time. In Niemann-Pick C1 (NPC1) protein-deficient lipidosis cells, the association of LDL-cholesterol with DRMs was enhanced and its transport to the plasma membrane was inhibited. In addition, the NPC1 protein was normally recovered in detergent-soluble membranes and its association with DRMs was enhanced by lysosomal cholesterol loading. Moreover, lysosomal cholesterol deposition was kinetically paralleled by the sequestration of sphingolipids and formation of multilamellar bodies in late endocytic organelles. These results suggest that late endocytic organelles are normally raft-poor and that endocytosed LDL-cholesterol is efficiently recycled to the plasma membrane in an NPC1-dependent process. The cholesterol-sphingolipid accumulation characteristic to NPC disease, and potentially to other sphingolipidoses, causes an overcrowding of rafts forming lamellar bodies in the degradative compartments.

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Crosslinking assay to study a specific cargo-coat interaction through a transmembrane receptor in the secretory pathway v1

10.17504/protocols.io.b3d9qi96 ◽

2022 ◽

Author(s):

Javier Manzano-Lopez†* ◽

Sofia Rodriguez-Gallardo† ◽

Susana Sabido-Bozo† ◽

Alejandro Cortes-Gomez ◽

Ana Maria Perez-Linero ◽

...

Keyword(s):

Protein Interactions ◽

Secretory Pathway ◽

Protein Complexes ◽

Secretory Protein ◽

Extracellular Proteins ◽

Transient Nature ◽

Transport Vesicles ◽

System P ◽

Cargo Receptor ◽

Cargo Proteins

Intracellular trafficking through the secretory organelles depends on transient interactions between cargo proteins and transport machinery. Cytosolic coat protein complexes capture specific luminal cargo proteins for incorporation into transport vesicles by interacting with them indirectly through a transmembrane adaptor or cargo receptor. Due to their transient nature, it is difficult to study these specific ternary protein interactions just using conventional native co-immunoprecipitation. To overcome this technical challenge, we have applied a crosslinking assay to stabilize the transient and/or weak protein interactions. Here, we describe a protocol of protein cross-linking and co-immunoprecipitation, which was employed to prove the indirect interaction in the endoplasmic reticulum of a luminal secretory protein with a selective subunit of the cytosolic COPII coat through a specific transmembrane cargo receptor. This method can be extended to address other transient ternary interactions between cytosolic proteins and luminal or extracellular proteins through a transmembrane receptor within the endomembrane system.

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Crosslinking assay to study a specific cargo-coat interaction through a transmembrane receptor in the secretory pathway v1

10.17504/protocols.io.bytapwie ◽

2021 ◽

Author(s):

Javier Manzano-Lopez † ◽

Sofia Rodriguez-Gallardo † ◽

Susana Sabido-Bozo ◽

Ana Maria Perez-Linero ◽

Rafael Lucena ◽

...

Keyword(s):

Protein Interactions ◽

Secretory Pathway ◽

Protein Complexes ◽

Secretory Protein ◽

Extracellular Proteins ◽

Transient Nature ◽

Transport Vesicles ◽

System P ◽

Cargo Receptor ◽

Cargo Proteins

Intracellular trafficking through the secretory organelles depends on transient interactions between cargo proteins and transport machinery. Cytosolic coat protein complexes capture specific luminal cargo proteins for incorporation into transport vesicles by interacting with them indirectly through a transmembrane adaptor or cargo receptor. Due to their transient nature, it is difficult to study these specific ternary protein interactions just using conventional native co-immunoprecipitation. To overcome this technical challenge, we have applied a crosslinking assay to immobilize the transient and/or weak protein interactions. Here, we describe a protocol of protein cross-linking and co-immunoprecipitation, which was employed to prove the indirect interaction in the endoplasmic reticulum of a luminal secretory protein with a selective subunit of the cytosolic COPII coat through a specific transmembrane cargo receptor. This method can be extended to address other transient ternary interactions between cytosolic proteins and luminal or extracellular proteins through a transmembrane receptor within the endomembrane system.

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Analysis of IFITM-IFITM Interactions by a Flow Cytometry-Based FRET Assay

International Journal of Molecular Sciences ◽

10.3390/ijms20163859 ◽

2019 ◽

Vol 20 (16) ◽

pp. 3859 ◽

Cited By ~ 4

Author(s):

Michael Winkler ◽

Florian Wrensch ◽

Pascale Bosch ◽

Maike Knoth ◽

Michael Schindler ◽

...

Keyword(s):

Antiviral Activity ◽

Protein Interactions ◽

Viral Entry ◽

Cellular Localization ◽

Fluorescent Protein ◽

Fluorescent Proteins ◽

Yellow Fluorescent Protein ◽

Resonance Energy Transfer ◽

Resonance Energy ◽

Protein Protein Interactions

The interferon-induced transmembrane proteins 1–3 (IFITM1–3) inhibit host cell entry of several viruses. However, it is incompletely understood how IFITM1–3 exert antiviral activity. Two phenylalanine residues, F75 and F78, within the intramembrane domain 1 (IM1) were previously shown to be required for IFITM3/IFITM3 interactions and for inhibition of viral entry, suggesting that IFITM/IFITM interactions might be pivotal to antiviral activity. Here, we employed a fluorescence resonance energy transfer (FRET) assay to analyze IFITM/IFITM interactions. For assay calibration, we equipped two cytosolic, non-interacting proteins, super yellow fluorescent protein (SYFP) and super cyan fluorescent protein (SCFP), with signals that target proteins to membrane rafts and also analyzed a SCFP-SYFP fusion protein. This strategy allowed us to discriminate background signals resulting from colocalization of proteins at membrane subdomains from signals elicited by protein–protein interactions. Coexpression of IFITM1–3 and IFITM5 fused to fluorescent proteins elicited strong FRET signals, and mutation of F75 and F78 in IFITM3 (mutant IFITM3-FF) abrogated antiviral activity, as expected, but did not alter cellular localization and FRET signals. Moreover, IFITM3-FF co-immunoprecipitated efficiently with wild type (wt) IFITM3, lending further support to the finding that lack of antiviral activity of IFITM3-FF was not due to altered membrane targeting or abrogated IFITM3-IFITM3 interactions. Collectively, we report an assay that allows quantifying IFITM/IFITM interactions. Moreover, we confirm residues F75 and F78 as critical for antiviral activity but also show that these residues are dispensable for IFITM3 membrane localization and IFITM3/IFITM3 interactions.

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Vesicular stomatitis virus glycoprotein, albumin, and transferrin are transported to the cell surface via the same Golgi vesicles.

The Journal of Cell Biology ◽

10.1083/jcb.97.6.1815 ◽

1983 ◽

Vol 97 (6) ◽

pp. 1815-1822 ◽

Cited By ~ 61

Author(s):

G J Strous ◽

R Willemsen ◽

P van Kerkhof ◽

J W Slot ◽

H J Geuze ◽

...

Keyword(s):

Vesicular Stomatitis Virus ◽

Intracellular Transport ◽

Intracellular Localization ◽

Protein A ◽

Secretory Protein ◽

Hepatoma Cells ◽

Secretory Proteins ◽

Human Hepatoma Cells ◽

Transmembrane Glycoprotein ◽

Vesicular Stomatitis

Human hepatoma cells, infected by vesicular stomatitis virus, offer a good system to study simultaneously the intracellular localization of a well defined transmembrane glycoprotein (VSV-G), a secretory glycoprotein (transferrin), and a nonglycosylated secretory protein (albumin). We used monospecific antibodies in combination with 5- and 8-nm colloidal gold particles complexed with protein A to immunolabel these proteins simultaneously in thin frozen sections of hepatoma cells. VSV-G, transferrin, and albumin are present in the same rough endoplasmic reticulum cisternae, the same Golgi compartments, and the same secretory vesicles. In the presence of the ionophore monensin intracellular transport is blocked at the trans cisternae of the Golgi complex, and VSV-G, transferrin, and albumin accumulate in dilated cisternae, which are apparently derived from the trans-Golgi elements. Glycoproteins, synthesized and secreted in the presence of monensin, are less acidic than those in control cultures. This is probably caused by a less efficient contact between the soluble secretory proteins and the membrane-bound glycosyltransferases that are present in the most monensin-affected (trans) Golgi cisternae.

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