Inhibition of Glucose Trimming with Castanospermine Reduces Calnexin Association and Promotes Proteasome Degradation of the alpha -Subunit of the Nicotinic Acetylcholine Receptor*

Steven H. KellerDagger , Jon Lindstrom§, and Palmer TaylorDagger

From the Dagger  Department of Pharmacology, University of California, San Diego, La Jolla, California 92093-0636 and the § Departments of Neurosciences and Pharmacology, University of Pennsylvania, Philadelphia, Pennsylvania 19104-6074

    ABSTRACT
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Abstract
Introduction
Materials & Methods
Results
Discussion
References

To identify factors involved in the expression of ligand-gated ion channels, we expressed nicotinic acetylcholine receptors in HEK cells to characterize roles for oligosaccharide trimming, calnexin association, and targeting to the proteasome. The homologous subunits of the acetylcholine receptor traverse the membrane four times, contain at least one oligosaccharide, and are retained in the endoplasmic reticulum until completely assembled into the circular arrangement of subunits of delta -alpha -gamma -alpha -beta to enclose the ion channel. We previously demonstrated that calnexin is associated with unassembled subunits of the receptor, but appears to dissociate when subunits are assembled in various combinations. We used the glucosidase inhibitor castanospermine to block oligosaccharide processing, and thereby inhibit calnexin's interaction with the oligosaccharides in the receptor subunits. Castanospermine treatment reduces the association of calnexin with the alpha -subunit of the receptor, and diminishes the intracellular accumulation of unassembled receptor subunit protein. However, treatment with castanospermine does not appear to alter subunit folding or assembly. In contrast, co-treatment with proteasome inhibitors and castanospermine enhances the accumulation of polyubiquitin-conjugated alpha -subunits, and generally reverses the castanospermine induced loss of alpha -subunit protein. Co-transfection of cDNAs encoding the alpha - and delta -subunits, which leads to the expression of assembled alpha - and delta - subunits, also inhibits the loss of alpha -subunits expressed in the presence of castanospermine. Taken together, these observations indicate that calnexin association reduces the degradation of unassembled receptor subunits in the ubiquitin-proteasome pathway.

    INTRODUCTION
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Abstract
Introduction
Materials & Methods
Results
Discussion
References

The nicotinic acetylcholine receptor is a prototype molecule of a family of ligand-gated ion channels, which include GABAA, glycine, and 5HT3 receptors (1, 2). Following binding by agonists to these receptors, a conformational change increases cation permeability through the central pore of the receptor, eliciting depolarization of the cell membrane (1, 2). Peptide backbones of each of the four subunits of the acetylcholine receptor transverse the membrane four times, and possess at least one Asn-X-Ser/Thr glycosylation signal (2, 3). The subunits are thought to undergo a maturation pathway which includes oligosaccharide attachment (4), formation of disulfide bonds (5-7), proline isomerization (8), and intersubunit contacts at specific interfaces (9-11). Members of this family of receptors are composed of a multisubunit complex of glycoproteins which are retained and assembled in the endoplasmic reticulum prior to transport to the cell surface (9, 12). Acetylcholine receptor subunits at the neuromuscular junction assemble into a circular orientation of subunits of delta -alpha -gamma -alpha -beta , to enclose the central ion channel (2, 13; but see Ref. 14).

The endoplasmic reticulum localized protein, calnexin, is associated with unassembled subunits of the acetylcholine receptor (15-17), but calnexin appears to be absent with combinations of assembled subunits (16). Connolly et al. (18) demonstrated that calnexin is associated with subunits of the GABAA receptor, indicating that calnexin association might be involved in the biogenesis of other multisubunit ion channels. Numerous investigations have established that calnexin associates primarily with monoglucosylated oligosaccharides, which are intermediates in the processing of nascent oligosaccharides or products of reglucosylation by the enzyme UDP-glucose:glycoprotein glucosyltransferase, and that treatment with the glucosidase inhibitor castanospermine can disrupt the interaction (reviewed in Refs. 19 and 20).

Using transient expression of acetylcholine receptor subunits in HEK cells, we find a role for calnexin association in reducing degradation of unassembled subunits by the proteasome, since treatment with castanospermine reduces the subunit-calnexin association and increases the polyubiquitination of the alpha -subunit. Additionally, co-treatment with proteasome inhibitors blocks the degradation. Although unassembled alpha -subunits are degraded at a rapid rate (5), treatment with glucosidase inhibitors substantially promotes degradation (4). Our data also indicate that castanospermine treatment does not cause the alpha -subunit to misfold, as detected by a conformationally sensitive antibody. Therefore, increased degradation by the proteasome appears to be independent of the nascent peptide undergoing misfolding in this system. In contrast, a recent study indicated that treatment of chick myotubes with castanospermine disrupts alpha -subunit folding and assembly (17). Our data also indicate that calreticulin and ERp57, the two other proteins known to have glycoprotein-associating properties similar to calnexin (19, 21), do not appear to be bound to the alpha -subunit.

Assembly with the delta -subunit reduces the degradation of the alpha -subunit when alpha - and delta -subunits are co-expressed in the presence of castanospermine, indicating that glucose trimming, calnexin association, assembly and entrance into the proteasome are linked in the expression of the receptor. Connections among these phenomena are also likely to be critical to the fidelity of expression of other multisubunit glycoproteins.

    MATERIALS AND METHODS
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Abstract
Introduction
Materials & Methods
Results
Discussion
References

Castanospermine Treatment and Transfections-- Castanospermine (Calbiochem, San Diego, CA) was solubilized in Dulbecco's modified Eagle's medium at a concentration of 100 µg/ml, and immediately added to 10-cm plates of cells. Cells were treated with castanospermine 2 h prior to transfection, transfected with receptor subunit cDNAs, allowed to grow for 16 h, or replenished with fresh castanospermine in Dulbecco's modified Eagle's medium and raised for another 24 h.

Transfections employed the calcium phosphate precipitation method, as described in Keller et al. (16). Generally, 15 µg of plasmid DNA encoding each receptor subunit were added to plates of cells, unless noted otherwise. In transfections where alpha - to delta -subunit ratios were varied, alpha -subunit cDNA was transfected at 15 µg of plasmid DNA/plate, and the mass of plasmid DNA encoding the delta -subunit was varied (Figs. 5 and 6).

Detergent Solubilization, Immunoprecipitation, Electrophoresis, and Western Blots-- In experiments involving immunoprecipitations with antibodies to calnexin, calreticulin, ERp57, and the receptor subunits, the solubilization buffer consisted of 0.5% CHAPS,1 150 mM NaCl, 1 mM CaCl2, 20 mM HEPES, pH 8.0, and the protease inhibitors: benzamidine, aprotinin, leupeptin, and pepstatin A. The characteristics of the antibodies used for these immunoprecipitations, mAb 35 or mAb 61 to precipitate the alpha -subunit, mAb 111 to precipitate the beta -subunit and mAb 137 to precipitate the delta -subunit, were described previously (22). Anticalnexin, antipolyubiquitin, and anti-calreticulin were purchased from Stressgen (British Columbia, Canada). Solubilization of cells and immunoprecipitations using anti-polyubiquitin were in 50 mM Tris-HCl, pH 8.0, 150 mM NaCl, 1 mM EDTA, 0.4% deoxycholate, 1% Nonidet P-40, 0.1% SDS, phenylmethanesulfonyl fluoride, N-ethylmaleimide, and the other protease inhibitors listed above. The ratio of solubilization buffer volume relative to the number of cell plates were the same for each sample within an experiment. Following solubilization, samples were centrifuged at 10,000 × g for 5 min. Dilution ratios for antibody in all immunoprecipitations were approximately 1:100.

Equivalent volumes of immunoprecipitated samples, consisting of approximately 5% of the total immunoprecipitated material, were loaded in each gel lane. All samples were resolved on 10% Novex gels (San Diego, CA) and transferred to nitrocellulose for Western blot detection. The antibodies used to detect the receptor subunits were mAb 210 for alpha , mAb 111 for beta , and mAb 137 for delta . The antibody to ERp57 was a gift from Dr. Jordan Holtzman (University of Minnesota). Calreticulin was detected on Western blots with the same antibody used in immunoprecipitations. All primary antibodies were diluted 1:1000 to probe Western blots, which were developed by chemiluminescent techniques (Pierce). Immunoprecipitation and Western blot experiments were replicated usually three or more times.

Proteasome Inhibitors-- Proteasome inhibitors were solubilized in Me2SO and added 3 h after transfection. Equivalent concentrations of Me2SO were added to untreated cells. The final concentration of Me2SO in a plate of cells was at most 0.3%. Cells were grown for an additional 16 h and then solubilized. The proteasome inhibitor benzyloxycarbonyl-Leu-Leu-phenylalaninal (Z-LLF-CHO) was obtained from Dr. F. Mercurio (Signal Pharmaceuticals, San Diego, CA) and used at a final concentration of 20 µM. MG-132 (carbobenzoxyl-leucinyl-leucinyl-leucinal) and lactacystin were purchased from Calbiochem (San Diego, CA) and used at 50 and 10 µM, respectively. Calpain inhibitor I (N-Ac-Leu-Leu-norleucinal; Calbiochem, San Diego, CA) was used at final concentration of 100 µM.

125I-alpha -Bungarotoxin Binding and Density Scans of Western Blots-- The snake toxin alpha -bungarotoxin (alpha -Bgt) binds to both unassembled and assembled alpha -subunits, whereas carbamoylcholine recognizes only alpha -subunits assembled with gamma -, delta -, or epsilon -subunits (10). Transfected and untransfected cells were permeabilized in a 0.1% saponin buffer (11), exposed to an excess of 125I-alpha -bungarotoxin (125I-alpha -Bgt) for 3 h, washed, and gamma -radiation was counted. The binding of 125I-alpha -Bgt to untransfected cells was subtracted from its binding to transfected cells. Data were standardized to the average of 125I-alpha -Bgt bound to cells untreated with castanospermine. Bands on Western blots were scanned with Deskscan (Hewlett Packard) and integrated with the program Collage (Fotodyne, New Berlin, WI).

    RESULTS
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Abstract
Introduction
Materials & Methods
Results
Discussion
References

Castanospermine Diminishes Accumulation of alpha -, beta -, and delta -Subunits in the Cell, without Generally Influencing the Accumulation of Other Cellular Proteins-- Cells were treated with the glucosidase inhibitor castanospermine, to identify roles for glucose trimming in the biogenesis of acetylcholine receptors expressed in HEK cells. Treatment with castanospermine, prior to and during the transfection period, inhibits the glucosidase I and glucosidase II enzymes, leaving oligosaccharides capped with three glucose residues. Castanospermine treatment, therefore, maintains larger sized oligosaccharides which are attached to glycoproteins confined to the endoplasmic reticulum. Since unassembled receptor subunits and alpha -delta dimers are retained intracellularly (23, 24), treatment with castanospermine should maintain larger oligosaccharides attached to the receptor subunits. A side reaction, which may result from a residual fraction of glucosidase enzymes remaining active, is that, nascent oligosaccharide chains whose glucosyl residues have been trimmed, in turn, become reglucosylated by UDP-glucose:glycoprotein-dependent glucosyltransferase. Reglucosylated receptor subunits may accumulate transiently because most glucosidase enzymes are inhibited (20).

Cells were untreated or treated with castanospermine prior to transfection with cDNAs encoding the alpha -, beta -, or delta -subunits. Following detergent solubilization, receptor protein was immunoprecipitated, resolved on gels, transferred to nitrocellulose and detected with appropriate antibodies. The Western blot in Fig. 1A demonstrates that castanospermine decreases the migration in gels of the alpha - (compare lanes 1 to 2), beta - (lanes 3 to 4), and delta -subunits (lanes 5 and 6), indicating untrimmed oligosaccharides predominate. The delta -subunit often appears as a doublet when resolved toward the bottom of a gel, which is presumably due to partial phosphorylation. Similarly, the alpha -subunit often appears as a doublet, with a faint unglycosylated lower molecular weight band and a more abundant higher molecular weight protein, which is glycosylated (25). gamma -Subunits were not included in these experiments due to the unavailability of the appropriate antibodies.


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Fig. 1.   Castanospermine treatment reduces the intracellular accumulation of alpha -, beta -, and delta -subunits but not a random sample of cellular proteins. A, cells were treated or untreated with castanospermine and transfected (TFT) separately with plasmid DNAs encoding alpha -subunits (lanes 1 and 2), beta -subunits (lanes 3 and 4), or delta -subunits (lanes 5 and 6). Detergent extracts were immunoprecipitated with antibodies specific for alpha  (mAb 61), beta  (mAb 111), or delta  (mAb 137), and receptor subunits were detected using mAb 210 for alpha -subunits, mAb 111 for beta -subunits, and mAb 137 for delta -subunits. Western blots were developed with chemiluminescent techniques. Equivalent volumes were loaded in each lane, consisting of approximately 5% of the immunoprecipitation mixture. Note in this and all subsequent blots that castanospermine treatment decreases slightly the mobilities of the receptor subunit bands, consistent with inhibition of glucose trimming. B, HEK cells were untreated (lanes 1 and 3) or treated with 100 µg/ml CST (lanes 2 and 4), grown for 18 h, cells were washed and detergent extracts were resolved in gels. Gels were either developed with Coomassie Blue stain (lanes 1 and 2) or protein was transferred to nitrocellulose and exposed to a high concentration of antimouse IgG-peroxidase to detect a random sample of cellular proteins (lanes 3 and 4). Equivalent volumes of detergent extract were loaded in each lane.

The banding densities in Western blots of alpha -, beta -, and delta -subunits are significantly diminished when expressed in castanospermine (Fig. 1A), indicating that the intracellular accumulations of these unassembled subunits are reduced. Although treatment with castanospermine at 100 µg/ml diminishes the accumulation of receptor protein, and presumably other glycoproteins, it does not influence the accumulation of most cellular proteins detected with a general stain or antibody (Fig. 1B). To establish this, untransfected cells were treated or untreated with castanospermine, and grown in a similar manner to transfected cells. Cells were harvested, washed 3 × in phosphate-buffered saline, and solubilized in the 0.5% CHAPS buffer as described earlier. Samples were resolved in gels, which were then stained with Coomassie Blue (Fig. 1B, lanes 1 and 2). Other samples were resolved in gels, transferred to nitrocellulose, and exposed to an excess of anti-rat IgG-conjugated peroxidase to detect cellular proteins nonspecifically (Fig. 1B, lanes 3 and 4). Proteins of similar banding densities align in the gels (Fig. 1B), indicating that the loss of acetylcholine receptor protein observed in Fig. 1A, is not due to a general reduction in protein synthesis caused by castanospermine treatment.

Polyubiquitinated alpha -Subunits Accumulate when Cells Are Treated with Proteasome Inhibitors-- To identify mechanisms which regulate receptor subunit degradation, experiments were designed to ascertain whether treatment with castanospermine increases conjugation of polyubiquitin to alpha -subunits. Cells were treated or untreated with castanospermine, transfected with cDNA encoding the alpha -subunit, and maintained in the presence of proteasome inhibitors: calpain inhibitor I and benzyloxycarbonyl-Leu-Leu-phenylalaninal (Z-LLF-CHO; 26). Calpain inhibitor I and Z-LLF-CHO were used in this experiment, because other investigations have demonstrated their efficacy for detecting the conjugation of polyubiquitin chains to proteins (27, 28). Detergent extracts were immunoprecipitated with an antibody to polyubiquitin, and Western blots were developed with mAb 210 to detect alpha -subunits (Fig. 2). The appearance of a characteristic ladder pattern near the top of the gel indicates that the proteins are polyubiquitinated (27-30). A high molecular weight ladder pattern is observed when alpha -subunits are expressed in the presence of castanospermine (Fig. 2A, lane 2), indicating that the alpha -subunits become polyubiquitinated. In comparison, alpha -subunits expressed in the absence of castanospermine are also polyubiquitinated, but the high molecular weight ladder pattern is fainter (Fig. 2A, compare lanes 1 and 2). The high molecular weight pattern is absent when Z-LLF-CHO is omitted in the experiment (Fig. 2B); this finding indicates that treatment with Z-LLF-CHO inhibits the degradation of polyubiquitinated alpha -subunits in the proteasome, thereby allowing the conjugated intermediates to accumulate. Treatment with calpain inhibitor I alone does not lead to the detection of polyubiquitinated alpha -subunits.


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Fig. 2.   A, castanospermine treatment enhances polyubiquitination of the alpha -subunit. Cells were incubated with or without castanospermine, and transfected with plasmid DNA encoding the alpha -subunit. All cells were treated with the proteasome inhibitors: calpain inhibitor I (CI) and Z-LLF-CHO. Extracts were immunoprecipitated with an antibody to polyubiquitin and the Western blot was developed with mAb 210, which detects the alpha -subunit. B, similar experiment to that described in A, but Z-LLF-CHO was omitted.

In other experiments with proteasome inhibitors, treatment with 50 µM MG-132 resulted in the detection of a distinct, but fainter high molecular weight ladder pattern compared with that observed with Z-LLF-CHO treatment; the density of the high molecular weight ladder pattern was also enhanced when cells were treated with castanospermine (data not shown).

Treatment with the Proteasome Inhibitors MG-132 or Lactacystin Inhibits the Degradation of alpha -Subunits-- To further characterize the mechanisms of degradation, cells were treated with the proteasome inhibitors lactacystin or MG-132, to examine whether degradation of alpha -subunits is reduced. Lactacystin is a irreversible inhibitor which binds specifically to the proteasome, as demonstrated by affinity labeling and peptide sequencing (31). MG-132 is a congener of Z-LLF-CHO, also a peptide-aldehyde that blocks the proteolytic activities of the proteasome (32). Cells were treated or untreated with castanospermine, transfected with the same plasmid DNA transfection mixture in all plates, and then treated or untreated with a proteasome inhibitor. Following an incubation period, cells were solubilized, and alpha -subunits were immunoprecipitated and detected on Western blots. As displayed in Fig. 3, lanes 3 and 4, and in previous experiments, treatment with castanospermine results in a loss of alpha -subunit protein; however, inclusion of lactacystin diminishes the loss of alpha -subunit protein (Fig. 3, lanes 1 and 2). Similar results were obtained with MG-132 (Fig. 4C, lanes 3 and 4). These data indicate that alpha -subunits, which may have been polyubiquitinated and subjected to isopeptidase activity (33), are degraded in the proteasome in cells treated with castanospermine.


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Fig. 3.   Lactacystin, a selective inhibitor of the proteasome, inhibits the degradation of alpha -subunits expressed in the presence of castanospermine. Cells were treated (+) or untreated (-) with CST, transfected with plasmid DNA encoding the alpha -subunit, treated (+) or untreated (-) with 10 µM lactacystin (LAC); an equivalent concentration of Me2SO was added to untreated cells, since LAC was solubilized in Me2SO. Samples were immunoprecipitated with mAb 61 and the Western blot developed with mAb 210. Equivalent numbers of cells were solubilized and subjected to immunoprecipitation and equivalent volumes were loaded in lanes, which consisted of approximately 5% of the total sample.


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Fig. 4.   Characteristics of calnexin recognition of alpha -subunits. A, cells were treated or untreated with CST and transfected (TFT) with 15 µg of plasmid DNA encoding the alpha -subunit or also co-transfected with 15 µg of plasmid DNA encoding the delta -subunit. Cells were not treated with a proteasome inhibitor. Sequential immunoprecipitation (IP to:) was first to calnexin (c), followed by immunoprecipitation of the unbound material with anti-alpha (mAb 61). Lanes 1 and 3, 2 and 4, 5 and 7, and, 6 and 8 are pairs of sequentially immunoprecipitated samples. The Western blot was developed with mAb 210 to detect alpha -subunits. The density ratios were calculated by scanning and integrating the density of alpha -subunit bands on the Western blot and dividing the CST-treated sample by the CST-untreated sample for alpha -subunits precipitated by one of the antibodies. B, similar to A, except cells were transfected with 3.0 µg of plasmid DNA encoding the alpha -subunit to reduce expression levels: cells were also treated with lactacystin. C, similar to A, except cells were treated with 50 µM MG-132. Blot was exposed to film 10 times longer than in A and B.

Treatment with lactacystin does not appear to enhance the accumulation of alpha -subunits expressed in the absence of castanospermine (Fig. 3, compare lanes 1 and 3), at a concentration of 10 µg/ml and 16 h of incubation. The degradation rate for alpha -subunits may be substantially lower when expressed in the absence of castanospermine, preventing detection of an enhanced accumulation in cells not treated with castanospermine. In support of a substantially lower degradation rate for alpha -subunits expressed in the absence of castanospermine, the conjugation of polyubiquitin chains is substantially reduced when alpha -subunits are expressed without castanospermine (Fig. 2A, compare lane 1 to 2).

To examine whether alpha -subunits are more prone to aggregate in cells treated with castanospermine, and whether this contributes to the loss of alpha -subunits, we analyzed insoluble fractions following detergent solubilization of cells. Cells were solubilized in the 0.5% CHAPS buffer described above, subjected to low speed centrifugation (5 min, 2,000 × g), and the resulting supernatant was subjected to high speed centrifugation (30 min, 16,000 × g). Western blots, of insoluble materials in the final fraction, displayed equivalently dense alpha -subunit bands in samples treated or untreated with castanospermine (data not shown). Therefore, we were unable to establish aggregation as a factor contributing to the loss of alpha -subunit protein expressed in the presence of castanospermine.

Treatment with Castanospermine Disrupts an Interaction between Calnexin and the alpha -Subunit-- To ascertain whether glucose trimming influences interactions between calnexin and alpha -subunits, cells were treated with castanospermine, and then transfected with various amounts of plasmid DNA encoding the alpha -subunit (Fig. 4). In some experiments, cells were also treated with proteasome inhibitors to reduce degradation and to facilitate the distinction between altered recognition by calnexin from increased degradation. Sequential immunoprecipitations were conducted with an antibody to calnexin (c), followed by immunoprecipitation of the unbound material with an anti-alpha - subunit antibody (mAb 61), to assess the extent of calnexin-alpha -subunit recognition. In Fig. 4, sequentially precipitated alpha -subunits are displayed, with lane 1 in sections A-C displaying alpha -subunits bound to calnexin, and lane 3 exhibiting the alpha -subunits not cleared with calnexin; likewise, lane 2 in sections A-C displays alpha -subunits bound to calnexin and lane 4 exhibits alpha -subunits not cleared with calnexin. Densities of alpha -subunit bands were quantified, and density ratios for alpha -subunits expressed in the presence relative to the absence of castanospermine were calculated. Each histogram bar was calculated separately for alpha -subunits precipitated with anti-calnexin or anti-alpha -subunit antibodies; for example, in Fig. 4, A-C, the histogram bars designated TFT: alpha  and IP to: c, were calculated for alpha -subunits co-immunoprecipitated with calnexin by anti-calnexin antibody, by dividing the band densities for alpha -subunits expressed in the presence (shown in lane 2) and absence of castanospermine (shown in lane 1). Similarly, the histogram bar designated as TFT: alpha  and IP to: alpha , was calculated for alpha -subunits immunoprecipitated with anti-alpha -subunit antibody, by dividing the band densities for alpha -subunits expressed in the presence and absence of castanospermine (displayed in lane 3). A comparison in the density ratios for alpha -subunits co-immunoprecipitated with calnexin relative to those immunoprecipitated with anti-alpha -antibody provides an estimate of the extent of calnexin-alpha -subunit recognition.

When cells are transfected with cDNA encoding the alpha -subunit at 15 µg of plasmid DNA/plate and are not treated with proteasome inhibitors, high levels of expression are observed, as evidenced by dense alpha -subunit bands for relatively short exposures of the blot to film (Fig. 4A, lanes 1-4). The density ratios for alpha -subunit bands (+CST/-CST) are similar when co-immunoprecipitated with calnexin or immunoprecipitated with anti-alpha subunit antibody (histogram, Fig. 4A), indicating treatment with castanospermine does not appear to repress the formation of the calnexin-alpha -subunit complex in this experiment. However, treatment with castanospermine causes a substantial loss of alpha -subunit protein (Fig. 4A, compare lanes 1 and 3 with 2 and 4), which may have included alpha -subunits that were not bound to calnexin because oligosaccharides were untrimmed.

When cells are co-transfected with cDNAs encoding the alpha - and delta -subunits at a 1:1 ratio of plasmid DNA masses, the association of calnexin with alpha -subunits is minimal (Fig. 4A, lanes 5 and 6), presumably because calnexin associates only with the small fraction of unassembled alpha -subunits present in these cells (16). Interestingly, when cells are treated with castanospermine and transfected with cDNAs encoding alpha - and delta -subunits at a 1:1 ratio of plasmid DNA masses, the loss of alpha -subunits in the cell is also minimal (Fig. 4A, compare lanes 7 and 8 to lanes 3 and 4). Since co-transfection of alpha - and delta -subunits at a 1:1 ratio of plasmid DNAs leads to the biogenesis of assembled alpha -delta dimers (11), these data indicate that the accumulation of assembled alpha -subunits is not impacted as significantly by aberrant glucose trimming. Data displayed in Fig. 4A also appear to indicate that calnexin association is more highly dependent on the extent of alpha -subunit assembly than treatment with castanospermine. This is evident because the alpha -subunit band isolated from cells co-transfected with plasmid DNAs encoding alpha - and delta -subunits, and co-immunoprecipitated with calnexin (Fig. 4A, lane 6), is attenuated relative to the alpha -subunit band isolated from cells expressing only alpha -subunits (Fig. 4A, lane 2). The assembly of alpha - and delta -subunits as dimers may occlude the association sites for calnexin.

In contrast to the above results, when receptor expression is lowered by transfection of 3 µg of plasmid DNA/plate encoding the alpha -subunit, and alpha -subunit degradation is reduced by treating cells with 10 µM lactacystin, the impaired glucose trimming by castanospermine appears to partially inhibit the formation of the alpha -subunit-calnexin complex (Fig. 4B). Treatment with castanospermine diminishes the fraction of alpha -subunits co-immunoprecipitated with calnexin (Fig. 4B, compare lanes 1 and 2), relative to alpha -subunits immunoprecipitated with anti-alpha -subunit antibody (Fig. 4B, compare lanes 3 and 4; histogram), illustrating an interaction between calnexin and the oligosaccharide on the alpha -subunit under these experimental conditions. Treatment with castanospermine similarly reduced the association of calnexin with alpha -subunits in cells transfected with 1.5 µg of plasmid DNA encoding the alpha -subunit, and treated with 10 µM lactacystin (data not shown).

Interactions between calnexin and the alpha -subunit oligosaccharide is further evidenced when alpha -subunits are expressed in the presence of 50 µM MG-132 (Fig. 4C). In this experiment, treatment with castanospermine appears to reduce substantially the ability of calnexin to associate with the alpha -subunit (Fig. 4C, lane 2), although alpha -subunits were readily detected in these cells (Fig. 4C, lane 4). The accumulation of alpha -subunits in cells was low in this experiment, since a 10-fold increase in the exposure time of this blot to film was necessary to detect a alpha -subunit band of comparable density. With this longer exposure, background protein bands are manifest in this experiment.

Recognition by calnexin of an appropriately trimmed oligosaccharide in the alpha -subunit becomes apparent in experiments using proteasome inhibitors, because the degradation of alpha -subunits not bound to calnexin and recovered by immunoprecipitation with anti-alpha -subunit antibody is reduced. Lowering receptor subunit expression may further facilitate the ability to detect an interaction between calnexin and an appropriately trimmed oligosaccharide in the alpha -subunit, by diminishing the probability for lower affinity interactions between polypeptide segments of calnexin and the receptor subunit. In summary, when expression levels are low and degradation is inhibited with proteasome inhibitors, an interaction between the alpha -subunit oligosaccharide and calnexin becomes apparent. However, additional interactions between calnexin and the alpha -subunit polypeptide backbone are also evident, especially when expression levels are high.

Assembly with delta -Subunits Reduces the Loss of alpha -Subunits Expressed in the Presence of Castanospermine-- To examine whether alpha -subunit assembly with the delta -subunit ameliorates the loss of alpha -subunits expressed in the presence of castanospermine, the mass of cDNA encoding the alpha -subunit was kept constant at 15 µg of plasmid DNA/plate and the plasmid DNA encoding the delta -subunit was transfected at two different ratios to alpha -subunit. Accumulation of alpha -subunits was measured using 125I-alpha -Bgt binding to permeabilized cells (Fig. 5): 125I-alpha -Bgt binding was also quantified in a similar manner with untransfected cells. Standardized values for 125I-alpha -Bgt binding are displayed in Fig. 5, where alpha -toxin binding to untransfected cells is subtracted from the values in transfected cells.


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Fig. 5.   Increasing the mass of plasmid DNA encoding the delta -subunit in the transfection increases the accumulation of alpha -subunits when subunits are coexpressed in the presence of castanospermine. Accumulation of folded alpha -subunits in the absence (-) or presence (+) of CST is measured by 125I-alpha -Bgt binding to permeabilized cells. alpha :delta ratios refer to the masses of plasmid DNAs in the transfection mixture, where the amount of plasmid DNA encoding the alpha -subunit is kept constant at 15 µg of DNA/plate and plasmid DNA encoding the delta -subunit is varied. Radioactivity (cpm) is standardized to the binding of 125I-alpha -Bgt to untransfected cells, and each histogram bar displays an average from two or three samples. The maximum counts/min are calculated as the average among samples untreated with castanospermine, determined separately for the two transfection ratios.

When the ratio of plasmid DNAs encoding the alpha - and delta -subunits is 1:2 in the transfection mixture, a 30% loss of alpha -subunit accumulation is observed in the castanospermine-treated cells (Fig. 5). However, when DNAs encoding the alpha - and delta -subunits are co-transfected at a 8:1 ratio, a 62% loss in the accumulation of alpha -subunits is evident in cells treated with castanospermine (Fig. 5). These data indicate that assembly of alpha -subunits with delta -subunits results in the stabilization of subunits coexpressed in the presence of castanospermine, and that the accumulation of assembled alpha -subunits is less dependent on the state of glucose trimming than is the accumulation of unassembled alpha -subunits.

Accumulation of alpha -delta Dimers Expressed in the Presence of Castanospermine Is Dependent on the Transfected Ratios of alpha - and delta -Subunit cDNAs-- To ascertain whether treatment with castanospermine and the stoichiometric ratios of cDNAs encoding alpha - and delta -subunits in the transfection influence the accumulation of alpha -delta dimers, cells were treated with castanospermine and co-transfected with plasmid DNAs encoding the alpha - and delta -subunits at ratios of 8:1 and 3:1. The mass of plasmid DNA encoding the alpha -subunit was kept constant at 15 µg of plasmid DNA/plate and the mass of plasmid DNA encoding the delta -subunit was varied. The alpha -subunit was immunoprecipitated with anti-alpha -antibody (mAb 61), and the Western blot was developed with antibodies to the alpha - and delta -subunits (mAb 210 and 137, respectively; Fig. 6A). The appearance of co-immunoprecipitated alpha - and delta -subunit bands appear to display correspondingly similar changes in density when coexpressed in the absence or presence of castanospermine, indicating that subunit assembly is not disrupted (Fig. 6A). The density of the delta -subunit band on the blot provides an indication of the accumulation of alpha -delta dimers. When cells are co-transfected with a large stoichiometric imbalance of subunits, using plasmid DNAs encoding alpha - and delta -subunits at a 8:1 ratio, there are significantly diminished alpha - and delta -subunit bands in the sample expressed in the presence of castanospermine, indicating alpha -delta dimers are less prevalent (Fig. 6A, compare lanes 1 to 2). However, treatment with castanospermine has a smaller impact on altering the density of alpha - and delta -subunit bands when plasmid DNAs are co-transfected at a 3:1 ratio, a closer stoichiometric balance of subunits (Fig. 6A, compare lanes 3 to 4). Similar results with respect to changes in the accumulation of assembled delta -subunits are displayed in Fig. 6B, in an experiment where plasmid DNAs encoding alpha  and delta  are co-transfected at ratios of 8:1 and 1:1. These data indicate that when alpha -subunits have a higher probability of contacting delta -subunits, glucose trimming has a smaller impact on the accumulation of alpha -delta dimers. These data also indicate that the ratios of nascent unassembled subunits and glucose trimming have a combined influence on the accumulation of assembled receptor subunits, which should ultimately dictate the expression levels of fully assembled receptors at the cell surface.


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Fig. 6.   The influence of castanospermine on the accumulation of alpha -delta subunit dimers depends on the transfection ratios of plasmid DNAs encoding the alpha - and delta -subunits. The transfected alpha :delta -subunit ratios refer to the masses of plasmid DNAs present in the transfection mixture, where the amount of plasmid DNA encoding the alpha -subunit is kept constant at 15 µg of DNA/plate and plasmid DNA encoding for the delta -subunit is varied. A, lanes 1 and 2 display samples transfected at a 8:1 ratio and lanes 3 and 4 display samples transfected at a 3:1 ratio of plasmid DNAs encoding the alpha - and delta -subunits. The numbers of cells, antibody dilutions for immunoprecipitations, and volumes loaded in each lane were the same among samples, and consisted of approximately 5% of the total sample. The Western blot was developed first with mAb 210 to detect the alpha -subunit and then reprobed with mAb 137 to detect the delta -subunit, and the exposures on films were overlaid to show alpha - and delta -subunits together. The delta -subunits displayed in the Western blot are assembled with alpha -subunits, since the immunoprecipitating antibody recognized the alpha -subunit (mAb 61). B, Western blot revealing assembled delta -subunits from a similar experiment as displayed in A, developed with mAb 137.

Calreticulin and ERp57 Association with alpha -Subunits Is not Detectable under Conditions where Calnexin Association Is Evident-- Similar to the binding properties of calnexin, calreticulin and ERp57 are thought to preferentially associate with newly synthesized glycoproteins which possess oligosaccharides capped with a single glucose residue (19, 21). Immunoprecipitation and Western blotting experiments were performed to ascertain whether calreticulin and ERp57 are associated with alpha -subunits. Calreticulin is expressed in HEK cells, as detected in a Western blot of a detergent extract (Fig. 7A, lane 1) and upon immunoprecipitation with an antibody to calreticulin (Fig. 7A, lane 4). However, co-immunoprecipitation of alpha -subunits with calreticulin was not appreciably detected (Fig. 7B, lane 2), although calreticulin was immunoprecipitated in this sample (Fig. 7A, lane 4), alpha -subunits were present in the extraction mixture (Fig. 7B, lane 4), and these conditions reveal co-immunoprecipitation of alpha -subunits with calnexin (Fig. 7B, lane 1). Association of alpha -subunits with calreticulin was also not detected when the detergent extract was immunoprecipitated with anti-alpha -antibody (mAb 61) and the Western blot developed with an antibody to calreticulin (data not shown). Experiments with the antibodies available to us indicate calnexin is more prevalently associated with alpha -subunits than is calreticulin.


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Fig. 7.   The alpha -subunit is not observed to associate appreciably with calreticulin (cr) and ERp57 under conditions which detect calnexin (c), yet all three proteins are present in HEK cells. Each sample represents equivalent numbers of cells, and equivalent volumes were loaded in gel lanes. A, Western blot developed with an antibody to calreticulin. Lane 1, Western blot of a detergent extract demonstrating calreticulin is present in HEK cells; lanes 2 and 3, immunoprecipitation using an antibody to calnexin without (lane 2) and with (lane 3) treatment of castanospermine; lane 4, immunoprecipitation using an antibody to calreticulin (TFT; transfected). B, cells were transfected with plasmid DNA encoding the alpha -subunit and the Western blot developed with an antibody to the alpha -subunit (mAb 210). Lane 1, detergent extract immunoprecipitated with an antibody to calnexin; lane 2, detergent extract immunoprecipitated with an antibody to calreticulin. This sample is also shown in A, lane 4, demonstrating immunoprecipitation of calreticulin; lane 3, immunoprecipitation of the unbound material using an antibody to the alpha -subunit (mAb 61; designated as c/61). This step followed the first immunoprecipitation to calnexin in lane 1; lane 4, immunoprecipitation of the unbound material using mAb 61, which followed the first immunoprecipitation to calreticulin in lane 2 (designated as cr/61). C, cells were transfected separately with plasmid DNAs encoding the alpha -subunit (lane 1) or the delta -subunit (lane 2), extracts were immunoprecipitated with antibodies to the receptor subunits (mAb 61 for alpha  and mAb 137 for delta ) and the Western blot was developed with an antibody to ERp57.

As with calreticulin, ERp57 was not observed to associate with alpha -subunits, by immunoprecipitating with mAb 61, and developing the Western blot with an antibody to ERp57 (Fig. 7C, lane 1). However, a delta -subunit-ERp57 association was detected by precipitating with a delta -subunit specific antibody (mAb 137), and developing the Western blot with the antibody to ERp57 (Fig. 7C, lane 2). The ERp57 antibody available to us does not immunoprecipitate ERp57 (data not shown), and therefore we were unable to use this antibody to co-immunoprecipitate the receptor subunits with ERp57, and detect the alpha -subunit on a Western blot. The delta -subunit has three oligosaccharide consensus sequences compared with one in the alpha -subunit, a difference that may contribute to the detection of the ERp57-delta -subunit association, but not an association with alpha -subunits.

Castanospermine Treatment Does Not Appear to Alter the Folding of alpha -Subunits, as Detected with a Conformationally Sensitive Antibody, whereas Assembly with delta -Subunits Increases the Fraction of Folded alpha -Subunits in the Cell-- We used mAb 35 reactivity to identify whether treatment with castanospermine influences the folding of unassembled alpha -subunits expressed in HEK cells. Cells were treated or untreated with castanospermine, and transfected with 15 µg of plasmid DNA/plate encoding the alpha -subunit. Sequential immunoprecipitations using mAb 35, which binds primarily to folded alpha -subunits (5), followed by an immunoprecipitation of the unbound material with mAb 61, which binds independently of conformation (5), were used to assess folding (Fig. 8A). Only a fraction of the alpha -subunit pool is recognized by mAb 35, indicating the alpha -subunit pool is predominantly unfolded when expressed in the absence of other subunits in HEK cells (Fig. 8A, lanes 1-4); this observation is consistent with previous observations in other cells (10, 34). An estimate of the fraction of folded alpha -subunits was obtained by measuring the density of alpha -subunit bands in Fig. 8 and dividing the respective mAb 35 density by the mAb 61 density (Fig. 8C). The fractions of alpha -subunits immunoprecipitated with mAb 35 relative to mAb 61 are similar when expressed in the absence or presence of castanospermine (22 and 29%, respectively; Fig. 8C). Within resolution limits of our assay, and the capacity of mAb 35 to detect folded subunits, glucose trimming does not appear to influence alpha -subunit folding.


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Fig. 8.   CST does not influence the folding of the alpha -subunit as detected by a conformation sensitive antibody (mAb 35); however, assembly with the delta -subunit increases the fraction of folded alpha -subunits. A, Western blot developed with an antibody to the alpha -subunit (mAb 210). Cells were transfected with plasmid DNA encoding the alpha -subunit or co-transfected with plasmid DNAs encoding the alpha - and delta -subunits at a 1:1 ratio of plasmid masses (15 µg of plasmid DNA/plate for each subunit). Sequential immunoprecipitations initially used mAb 35, which has a higher affinity for folded alpha -subunits, and then unbound material was immunoprecipitated with mAb 61. Both antibodies, at a concentration of 5 mg/ml, were diluted 1:100 prior to a 1.5-h immunoprecipitation. The intensity of the alpha -subunit band immunoprecipitated by mAb 35 relative to mAb 61 provides an indication of the fraction of folded alpha -subunits. B, same Western blot as in A, but reprobed with an antibody to delta  (mAb 137), indicating the relative amounts of assembled delta -subunits. Lanes 5-8 in B correspond to lanes 5-8 in A. C, quantitation of the fraction of folded alpha -subunits in the Western blot displayed in A, calculated as the ratio of densities for alpha -subunits immunoprecipitated with mAb 35 relative to alpha -subunits immunoprecipitated with mAb 61; alpha - and alpha + refer to cells transfected with plasmid DNA encoding the alpha -subunit, untreated or treated with castanospermine, respectively, and alpha delta - and alpha delta + refer to cells co-transfected with plasmid DNAs encoding the alpha - and delta -subunits, untreated and treated with castanospermine, respectively.

To examine whether assembly with delta -subunits influences the folding of alpha -subunits, plasmid DNAs encoding the alpha - and delta -subunits were co-transfected at a 1:1 ratio of DNA masses, sequential immunoprecipitations were performed with mAbs 35 and 61, and the extent of folding was quantified by density scans of Western blots. The Western blot was developed first with mAb 210 to detect alpha -subunits (Fig. 8A, lanes 5-8), and then reprobed with mAb 137 to detect assembled delta -subunits (Fig. 8B, lanes 5-8). A larger fraction of the alpha -subunit pool is immunoprecipitated with mAb 35 when alpha - and delta -subunits are coexpressed (Fig. 8A, compare lanes 1-4 to lanes 5-8), indicating alpha -subunits fold, or are maintained in a folded state, when assembled with delta -subunits. Moreover, treatment with castanospermine does not significantly alter the ratio of folded alpha -subunits when alpha - and delta -subunits are coexpressed (Fig. 8, A, lanes 5-8 and C). Fig. 8B displays delta -subunits assembled with alpha -subunits, since the same Western blot in Fig. 8A was reprobed with an antibody to delta -subunits (mAb 137). A larger fraction of delta -subunits are associated with alpha -subunits which are recognized by mAb 35 (Fig. 8, A and B, compare lane 5 with lane 6 and lane 7 with lane 8), further indicating that assembly promotes alpha -subunit folding.

MAb 35 displays a corresponding increase in affinity for folded alpha -subunits during maturation (5). The affinity of alpha -Bgt for the alpha -subunit also increases correspondingly with maturation (5). Since mAb 35 recognizes a region distinct from the primary contact sites of alpha -Bgt (22), it can be used as a global indicator for the folding of the extracellular domain of the alpha -subunit. At the dilutions and times for antibody incubations used in this study, a clear distinction in Western blot banding densities was observed for unassembled relative to assembled alpha -subunits, which were immunoprecipitated with mAb 35.

In summary, the data compiled in Fig. 8C indicate that, assembly with the delta -subunit increases the fraction of folded alpha -subunits which accumulate in cells. Therefore, the delta -subunit may play a chaperone-like role promoting the folding of the alpha -subunit. An alternative explanation for the observed enhancement in the accumulation of folded alpha -subunits, is that, folded alpha -subunits are more likely to assemble and alpha -delta complexes accumulate because they are more stable. However, our data indicate that the fraction of folded alpha -subunits is increased relative to the total alpha -subunit pool expressed in these cells.

We additionally sought to ascertain whether treatment with castanospermine disrupts the assembly of alpha - with delta -subunits, by co-transfecting plasmid DNAs encoding alpha - and delta -subunits and estimating the extent of assembly with differential ligand binding (16). The specific binding of 125I-alpha -Bgt in cells incubated in the presence of carbamoylcholine, which blocks alpha -subunits assembled with delta -, gamma -, or epsilon -subunits, estimates the accumulation of alpha -subunits which are unassembled and folded. To estimate the accumulation of assembled and folded alpha -subunits, the quantity of unassembled and folded alpha -subunits is subtracted from the total specific 125I-alpha -Bgt bound in cells (16). Therefore, the numerical ratio of unassembled alpha -subunits to assembled alpha -subunits, as estimated by 125I-alpha -Bgt binding, takes into account both subunit folding and assembly. Based on the mean of four samples for cells treated, and four samples for cells untreated with castanospermine, our data revealed similar ratios of unassembled alpha -subunits to assembled alpha -delta dimers (without castanospermine, 0.083; with castanospermine, 0.080). These nearly identical numerical values indicate that treatment with castanospermine does not significantly alter both the folding and assembly of alpha - and delta -subunits. Furthermore, Western blots of co-transfected alpha - and delta -subunits show by subunit mobility that castanospermine efficiently inhibits glucose trimming (Fig. 6A). However, coimmunoprecipitated alpha - and delta -subunit bands display correspondingly similar density changes for cells treated and untreated with castanospermine (Fig. 6A), further indicating that glucose trimming does not significantly impact alpha -delta subunit assembly. Similar results were obtained when plasmid DNAs encoding alpha - and delta -subunits were transfected at 1:1 ratios (data not shown).

    DISCUSSION
Top
Abstract
Introduction
Materials & Methods
Results
Discussion
References

Of the three proteins thought to be involved in the biogenesis of glycoproteins, and to associate primarily with glycoproteins possessing oligosaccharides capped with one glucose residue (19, 21), only calnexin was found to associate with the receptor alpha -subunits. Calreticulin and ERp57 could be associated with alpha -subunits in vivo, but the interaction was undetectable in vitro, by using antibodies available to us and techniques which readily detect calnexin in association with alpha -subunits. Based on data presented in this study, the processing events in receptor biosynthesis which are altered by castanospermine treatment appear to be related to calnexin association.

Recognition of alpha -subunits by calnexin appears to be rather complex, with calnexin displaying association to both oligosaccharide structures and the polypeptide backbone. Calnexin binding to the alpha -subunit oligosaccharide is dependent on oligosaccharide trimming, because castanospermine treatment reduces the interaction. The importance for oligosaccharide trimming in this interaction becomes apparent when expression levels are low, and degradation is inhibited with a proteasome inhibitor (Fig. 4, B and C). These observations may indicate that the calnexin-oligosaccharide interaction displays a higher affinity with unassembled subunits, than the calnexin-polypeptide interaction. In fact, several investigations have suggested that calnexin displays a sufficient affinity to bind directly to oligosaccharide structures irrespective of the polypeptide backbone (19, 35).

The additional interaction between calnexin and the alpha -subunit polypeptide backbone appears to be dependent on subunit assembly, because assembly with the delta -subunit reduces calnexin association, and this interaction is not significantly altered by castanospermine treatment (Fig. 4A, lanes 5-8). Subunit assembly may inhibit the calnexin-polypeptide interaction, because the newly formed contact interface between subunits occludes the lower affinity association with calnexin. Alternatively, alpha -subunits which fold upon assembly may bury an interface which is required for calnexin attachment.

In agreement with our observations that castanospermine increases receptor degradation, an earlier study with BC3H-1 cells showed that, treatment with the glucosidase inhibitor 1-deoxynojirimycin decreased the stability of unassembled alpha -subunits expressed from the endogenous gene (4). Investigations on other transmembrane spanning glycoproteins have also revealed a decreased stability of glycoproteins expressed under conditions which impair glucose trimming (36-38). In contrast, studies of secretory protein processing indicate that calnexin association correlates with the instability of these proteins (39, 40).

The ubiquitin-proteasome pathway appears to be involved in the degradation of alpha -subunits expressed in the presence of castanospermine, because polyubiquitinated alpha -subunits accumulate in cells treated with proteasome inhibitors. Moreover, the degradation of alpha -subunits is inhibited when cells are treated with the specific proteasome inhibitor lactacystin (31), localizing the proteasome as the site for the degradation. Several investigations have established that proteins embedded in the ER membrane are susceptible to degradation in the proteasome, with examples including the cystic fibrosis transmembrane conductance regulator (29, 41), major histocompatibility complex subunits (42-44), and T-cell receptor subunits (45). Treatment with proteasome inhibitors can result in the detection of conjugated polyubiquitin chains (29), and an enhanced accumulation of proteins which would otherwise be targeted for degradation (29, 45). Investigations on major histocompatibility complex subunits (42-44) and T-cell receptor alpha -subunits (45) have also revealed that degradation of misfolded or unassembled proteins follows a pathway which involves retrograde transport through the Sec61 protein translocator channel (43, 44), cytoplasmic deglycosylation, and degradation in the proteasome (43-45). The alpha -subunit of the acetylcholine receptor has numerous lysine residues positioned in its two cytoplasmic loops (i1-2 and i3-4); these and other lysines positioned at the cytoplasmic and luminal boundaries of the transmembrane domains, and in the extracellular domains, may serve as polyubiquitin attachment sites, which target receptor subunits to the proteasome.

Treatment with castanospermine may perturb the assembly pathway, where calnexin association is a critical step which stabilizes unassembled receptor subunits. Disruption of this interaction, and bi-directional motions of the alpha -subunit, may lead to increased exposure of ubiquitin attachment sites at the cytoplasmic boundary, and promote targeting of the subunit to the proteasome. Furthermore, the association of calnexin with the alpha -subunit may occlude the ability of the alpha -subunit-calnexin complex to move through a relatively narrow Sec61 channel (46). A low affinity interaction between calnexin and unassembled alpha -subunits, in the absence of artificially impaired glucose trimming with castanospermine, might release proteins to enter the degradative pathway. In support of the notion that retrograde transport is a component of the degradative pathway for acetylcholine receptor subunits, we have preliminary data indicating that treatment with castanospermine and proteasome inhibitors results in an enhanced accumulation of unglycosylated alpha -subunits.2

Ubiquitin-conjugating enzymes have been identified to reside on the cytoplasmic exposure of the ER membrane in yeast (47, 48), and attachment of ubiquitin chains is a requirement for efficient degradation via retrograde transport and proteasome hydrolysis (48). The presence of a homologous enzyme in HEK cells might conjugate ubiquitin molecules to sites on acetylcholine receptor subunits exposed just outside the cytoplasmic face of the ER membrane. In contrast, an attachment of calnexin to secretory proteins may result in their localization near to the ER membrane, and this may contribute to their destabilization. Secretory proteins which are positioned at the ER membrane may become dissociated from calnexin, translocated through the Sec61 channel, and degraded in the proteasome.

Assembly with delta -subunits may further stabilize the alpha -subunits, by constraining the folded conformation, increase tethering in position in the membrane, and physically inhibit the ability of the larger alpha -delta dimer complex from moving through the Sec61 channel. The juxtaposition of alpha - and delta -subunits may also limit the accessibility of the ubiquitin conjugating machinery to previously exposed lysine residues. The above hypotheses concerning the degradative pathway for receptor alpha -subunits are consistent with observations that: (a) calnexin dissociation diminishes the accumulation of receptor subunits, and (b) assembly of alpha -subunits with delta -subunits correlates with further folding and stabilization of alpha -subunits.

Our experiments indicate that castanospermine treatment does not significantly alter the folding of alpha -subunits, or the assembly of alpha -subunits with delta -subunits. Supportive data in two other investigations have also indicated that alpha -subunit folding and assembly are not significantly impacted by impaired glucose trimming (4, 49). In contrast, castanospermine treatment was observed to disrupt folding and assembly of alpha -subunits expressed in chick myotubes (17). This investigation also indicated that overexpression of calnexin, by transfection of a cDNA encoding calnexin, led to enhanced assembly and surface expression of alpha -subunits in COS and HEK cells (17).

Glucose trimming and calnexin association may have their greatest impact on the expression of multisubunit glycoprotein complexes when the translation product of any subunit is a minor component of the total protein embedded in the endoplasmic reticulum membrane, and there is a stoichiometric imbalance in the expression of each subunit. This hypothesis is consistent with the observation that the accumulation of alpha -delta dimers, which are expressed in the presence of castanospermine, is significantly diminished when delta -subunits are in a large stoichiometric deficiency to alpha -subunits. Using muscle cells, several investigations have revealed that endogenous acetylcholine receptor subunits are expressed in stoichiometric imbalances (24, 50, 51).

    ACKNOWLEDGEMENTS

We thank Dr. J. Holtzman for providing an antibody to ERp57 and Drs. J. DiDonato and F. Mercurio for providing Z-LLF-CHO.

    FOOTNOTES

* This work was supported by United States Public Health Service Fellowship NS09715 (to S. H. K.), National Institutes of Health Grant NS11323, MDA, and Smokeless Tobacco Research Council, Inc. grants (to J. L.), and United States Public Health Service Grant GM18360 (to P. T.).The costs of publication of this article were defrayed in part by the payment of page charges. The article must therefore be hereby marked "advertisement" in accordance with 18 U.S.C. Section 1734 solely to indicate this fact.

1 The abbreviations used are: CHAPS, 3-[(3-cholamidopropyl)dimethylammonio]-1-propanesulfonate; Bgt, bungarotoxin; CST, castanospermine; ER, endoplasmic reticulum; HEK, human embryonic kidney; Me2SO, dimethyl sulfoxide; LAC, lactacystin; Z-LLF-CHO, benzyloxycarbonyl-Leu-Leu-phenylalaninal; mAb, monoclonal antibody.

2 S. Keller, unpublished data.

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Abstract
Introduction
Materials & Methods
Results
Discussion
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