©1996 by The American Society for Biochemistry and Molecular Biology, Inc.
Control of -Glutamyl Transpeptidase Expression by Glucocorticoids in the Rat Pancreas
CORRELATION WITH GRANULE FORMATION (*)

(Received for publication, December 11, 1995; and in revised form, February 28, 1996)

Marie Noële Chobert (§) Gilles Grondin Arthur Brouillet Yannick Laperche Adrien R. Beaudoin

From the Institut National de la Santé et de la Recherche Médicale, Unité INSERM 99, Hôpital Henri Mondor, 94010 Créteil, France and Département de Biologie, Faculté des Sciences, Université de Sherbrooke, Sherbrooke, Québec J1K 2R1, Canada

ABSTRACT
INTRODUCTION
EXPERIMENTAL PROCEDURES
RESULTS
DISCUSSION
FOOTNOTES
ACKNOWLEDGEMENTS
REFERENCES

ABSTRACT

Glucocorticoids are known to promote the formation of zymogen granules in acinar cells of the exocrine pancreas in vivo as well as in vitro. To gain insight into the mechanism of this regulation, we studied the effects of glucocorticoids on the synthesis of two components of the secretory granule membrane, the glycoprotein 2 (GP-2) and the -glutamyl transpeptidase (GGT). It was demonstrated that following adrenalectomy, degranulation of pancreatic acinar cells is accompanied by a sharp decrease in GGT and GP-2 synthesis as measured by mRNA and protein accumulation. The decline of GGT synthesis was prevented by glucocorticoid replacement therapy, whereas GP-2 synthesis could be maintained with either glucocorticoid or estradiol treatment. These in vivo observations were corroborated and extended in an in vitro study using AR42J pancreatic cells. With this cell line, it was demonstrated that dexamethasone induces the formation of zymogen granules and the accumulation of a specific GGT transcript (mRNA III) by decreasing its degradation rate. At the same time, the GP-2 mRNA level was not modified by the hormonal treatment. These data demonstrate that glucocorticoids exert a positive control on the GGT expression in pancreatic cells at a post-transcriptional level. GGT, an enzyme of the glutathione metabolism, could play a significant role in protein packaging in secretory cells.


INTRODUCTION

In eukaryotic cells, newly synthesized secretory proteins are sequestered in the rough endoplasmic reticulum and delivered to the Golgi apparatus. At the trans-side of the Golgi, most of the secretory proteins are packaged into secretory granules, a storage compartment. Upon stimulation, the granules move to the cell apex and release their content by exocytosis(1, 2) .

Despite a considerable amount of progress in our understanding of the intracellular trafficking of secretory proteins, the mechanisms by which they are packaged and maintained in an osmotically inactive form in the zymogen granule (ZG) (^1)is unknown. Possible clues for the elucidation of these processes come from experiments which reported that adrenalectomy of male rats caused a marked depletion of ZG in the pancreas acinar cells, an effect which was reversed by treatment with the synthetic glucocorticoid, triamcinolone(3, 4) . It was also found that a dexamethasone treatment of the AR42J rat pancreatic cells induces the appearance of ZG(5) . These observations led us to the hypothesis that glucocorticoids were directly involved in the packaging of secretory proteins and ZG formation.

Glucocorticoids could influence the packaging of secretory proteins and ZG formation through the ZG membrane protein content. The latter membrane is a highly specialized membrane; it contains, roughly, 10 major proteins and shows a rather limited spectrum of polypeptides(6, 7) , with a significant overlapping composition to membranes from other exocrine glands, irrespective of the nature of stored proteins(8) . The glycoprotein 2 (GP-2) is one of the major components of this membrane; it is a glycosyl phosphatidylinositol-anchored protein (9, 10) that is released in the pancreatic ducts upon cleavage with a phosphatidylinositol-phospholipase. The released GP-2 polymerizes and forms a fibrillar network(11, 12) . The physiological role of GP-2 is not yet defined, but this fibrillar network may form a barrier to colonization of the pancreatic duct by intestinal bacteria. In addition, recent studies have shown that GP-2 shares some antigenic determinants and structural homology with a phospholipase A(2)(13) . -Glutamyl transpeptidase (GGT) is another glycoprotein component of the secretory granule membranes, which has been used as a marker to follow their isolation by subcellular fractionation(8) . In the exocrine pancreas, we localized GGT, which is a type II membrane protein, in the ZG membrane, the apical membrane and pancreatic juice (14) where it is associated with ``pancreasomes'' (12, 15) . GGT hydrolyzes glutathione, which may affect the disulfide bridges of the proteins with high cysteine content, like GP2, along the secretory pathway(16) . Biochemical and immunocytochemical observations have indicated that both GP-2 and GGT are continuously released by the pancreas acinar cell in the pancreatic juice, and, hence, a substantial fraction of these proteins do not follow its host membrane that recycles after exocytosis(11, 12, 15) . This implies a de novo synthesis of these proteins and their insertion into the recycled membrane as new granules form. If these proteins are essential for protein packaging and ZG formation, therefore, one could postulate an increase in their rate of synthesis when ZG formation is induced by glucocorticoids(4) .

The study of the expression of these two very different membrane proteins is now greatly facilitated as a result of cloning and sequencing of their respective cDNAs(10, 17) . In the rat, GGT is encoded by a single copy gene (18) transcribed into several mRNA species (mRNAs I to V) according to the tissues(19, 20, 21, 22, 23) . The GP-2 protein is also encoded by a single copy gene, but only one species of mRNA is transcribed(10, 24) . In this work, we show that in acinar cells, glucocorticoid treatment induces in parallel ZG formation and GGT expression. The GGT regulation occurs at a post-transcriptional level since glucocorticoids induce the accumulation of the GGT mRNA III transcript by decreasing its degradation. We also provide evidence that ZG formation can be induced independently of GP-2 expression.


EXPERIMENTAL PROCEDURES

Animals and Treatments

Male Sprague-Dawley rats, weighing approximately 200 g, were used for these experiments. The animals were maintained on 0.9% saline drinking solution in addition to standard lab chow. They were divided in four groups of 10 animals, 1) sham-operated, 2) adrenalectomized, 3) adrenalectomized with a dexamethasone replacement therapy, 4) adrenalectomized with an estradiol replacement therapy. The experiments lasted 5 days starting with surgery on day 0. The following day, the rats on a replacement therapy received the hormone for 4 days. The animals were fasted overnight prior to their sacrifice on the 5th day. For the glucocorticoid replacement therapy, the animals were given 0.09 mg of dexamethasone in propylene glycol (Organon, Toronto, Canada), and for the estradiol replacement therapy, the animals received 0.042 mg of estradiol in propylene glycol (Sigma) as daily subcutaneous injections. The rats were decapitated and the pancreases quickly excised. Small pieces of tissues chosen at random in different regions of the gland were immediately fixed for morphological observations or used for GGT assay or RNA preparation. Livers were also excised from 18-day-old fetuses and from adult rats. Kidneys were obtained from adult rats and mammary glands from lactating female rats.

Cell Culture

The AR42J pancreatic carcinoma cells (CRL 1492) were obtained from the ATCC (Rockville, MD). The cells were plated at a density of 1.5 times 10^6 cells per 10-cm dishes and grown for 4 days in modified Ham's F12 medium (Life Technologies, Inc., Cambridge, U. K.), supplemented with 10% fetal calf serum, 200 units/ml penicillin, 50 µg/ml streptomycin, and 0.5 µg/ml fungizone, before different periods of treatment by 10 or 100 nM dexamethasone. In some experiments, the anti-glucocorticoid RU-38486 (gift from Roussel-Uclaf, France) was added to the dexamethasone-treated cells at a 0.5 mM concentration. Cells were lysed directly into 1.5 ml of 4 M guanidium thiocyanate per dish for RNA extraction or washed two times in cold PBS and scraped for GGT assay, Western blot analysis, or nuclei purification.

Electron Microscopy

Cell pellets and pieces of pancreas tissues were processed for electron microscopy as described previously (4) .

GGT Assay

Tissues were homogenized in water with a Potter-Elvehjem, and AR42J cells were washed, scraped, and suspended in PBS. The GGT activity was determined according to Orlowski and Meister (25) and expressed as unit/mg protein. One unit corresponds to 1 µmol of product formed per min at 37 °C. Proteins were assessed according to Bradford(26) .

Western Blot Analysis of GP-2

Pancreases were homogenized with a Polytron homogenizer (Brinkman Instruments) in 45 mM Tris saline buffer, pH 7.6, and centrifuged at 700 times g for 15 min in a Beckman JA-20 rotor. Supernatants were decanted and centrifuged for 60 min at 100,000 times g in a Beckman S.W.41 rotor. The pellets were suspended in 5 mM Tris, 5% glycerol, pH 7.6. AR42J cells were washed and scraped in PBS; pellets were suspended in 1% SDS and boiled for 5 min. Proteins were estimated according to Bradford(26) . Samples (100 µg) were resuspended in loading buffer and separated by SDS-polyacrylamide gel electrophoresis according to Laemmli(27) . Proteins were stained with Coomassie Blue and GP-2 immunoblotting carried out as described previously(28) .

RNA Preparation

Total RNA was extracted from rat tissues or AR42J cells using the guanidium thiocyanate procedure(29) . Poly(A) RNA were obtained by two successive purifications on an oligo(dT) column as described previously(19) , or using the microspin oligo(dT) column (RNA-Flash from Bioprobe Systems, Montreuil-sous-bois, France) when the amount of total RNA was less than 2 mg.

Northern Blot Analysis

The poly(A) RNA samples were resolved on an 1.5% agarose denaturing gel, transferred onto a nylon membrane (Hybond N, Amersham, France), and hybridized to GGT and GP-2 probes as described previously(19) . Blots were also hybridized to a beta-actin probe to assess the amount of sample loaded on the gel.

The labeled GGT complementary RNA (cRNA) probes, which hybridize specifically to the GGT mRNA I (cRNA-17), mRNA II (cRNA-12), mRNA III (cRNA-3), or to all the GGT mRNA types (cRNA-139A), were synthesized by in vitro transcription of the GGT plasmids pGEM-17, pGEM-12, FL2, or pGEM4-139 as described elsewhere (19, 22) . These plasmids were linearized by NsiI (pGEM-17), HincII (pGEM-12), or SacI (FL2 and pGEM4-139) prior to their transcription from the T7 promoter in the presence of [alpha-P]UTP, except for FL2 which was transcribed from its SP6 promoter. The GP-2 cRNA probe was obtained from a GP-2 recombinant plasmid (10) kindly provided by Dr. C. Rindler. The coding sequence, from the nucleotide 174 to the nucleotide 1607, was subcloned into pGEM-4 (Promega, Madison) and digested by EcoRI and BamHI. The recombinant plasmid was then linearized by EcoRI and transcribed from its T7 promoter. The beta-actin probe was obtained by labeling the 800-bp HindIII-KpnI cDNA fragment(30) , using the megaprime labeling kit (Amersham, France) in the presence of 50 µCi of [alpha-P]dATP.

Run-on Experiments

Nuclei were prepared as described previously(31) . Nascent RNA transcripts were labeled with [alpha-P]UTP, isolated, and quantitated according to Antras et al.(32) . The labeled RNA (10 times 10^6 cpm) was hybridized to an Hybond membrane where either 10 µg of control pGEM-3Zf(+) DNA (Promega, Madison) or 3 µg of GP-2 cDNA, 2 µg of amylase cDNA, and 1.7 µg of a 470-bp GGT genomic sequence have been immobilized. This latter 470-bp GGT sequence was obtained from the plasmid pGEM-III(22) ; it contains the 58 nucleotides at the 3`end of the GGT mRNA III leader exon and extends 412 nucleotides downstream in the first intron. The 0.9-kb amylase cDNA sequence cloned into the plasmid pBR322 (33) was kindly provided by Dr. R. J. MacDonald. After hybridization, the blots were autoradiographed, and densitometric quantification of the signals was carried out using a Laser densitometer Ultroscan XL (Pharmacia Biotech, Inc.).

Measurement of the GGT mRNA III Degradation Rate

The AR42J cells were incubated for 48 h in the presence or in the absence of 100 nM dexamethasone prior to the addition of actinomycin D (1.25 µg/ml) for different periods of time. The total RNA was extracted, and aliquots (10-40 µg) were used to assess the amount of GGT mRNA III-specific sequences by an RNase protection assay using the Ambion kit (Clinisciences, Montrouge, France). The cRNA-3 probe (362 bases) was transcribed from the GGT plasmid FL2 linearized by EcoRI. The probe was purified on a 5% acrylamide, 8 M urea gel and eluted; 250,000 cpm of labeled cRNA were coprecipitated with each RNA sample. The pellets were resuspended in 80% deionized formamide, 100 mM sodium citrate, pH 6.4, 300 mM sodium acetate, pH 6.4, 1 mM EDTA. Hybridization was performed overnight at 55 °C. The hybridization products were digested by the RNase A and T1 for 30 min at 37 °C, treated as described in the kit procedure, and loaded on a 5% acrylamide, 8 M urea gel. The gel was run for 2 h at 50 watts, dried, and autoradiographed. Densitometric quantification was performed using a Laser densitometer Ultroscan XL (Pharmacia). Films were exposed for different periods of time in order to measure the intensity of the signal in a linear range.


RESULTS

Morphological Examination

As illustrated by representative micrographs (Fig. 1, A-D), a decrease in the number of ZG was observed in the pancreatic acinar cells of adrenalectomized rats (Fig. 1B) as compared with the number found in cells from control animals (Fig. 1A). There is no noticeable difference between the pancreases of the adrenalectomized group (Fig. 1B) and those of animals receiving estradiol as a replacement therapy (Fig. 1C). In contrast, the animals of the adrenalectomized group that received a replacement therapy with dexamethasone (Fig. 1D) exhibited an increase in the number of ZG in the pancreas, as compared with the controls. In control AR42J cells, there were only few small size granules (Fig. 2A). Dexamethasone treatment induces the appearance of ZG of different sizes (Fig. 2B).


Figure 1: Effect of dexamethasone and estradiol on granulation of rat pancreatic acinar cells (800 times magnification). A, sham-operated rats. Zymogen granules are numerous on the luminal side of the acini. B, adrenalectomized rats. The number of granules decreases in each cell. C, adrenalectomized rats treated by estradiol. The hormone does not modify the degranulation induced by adrenalectomy. D, adrenalectomized rats treated by glucocorticoids. Regranulation is observed in all acini; the number of zymogen granules is higher than in control cells from sham-operated rats.




Figure 2: Effect of dexamethasone on granulation of AR42J cells. A, control AR42J cells. Few ZG are found in these cells where nucleus (NU) occupy a large volume (times 9900). B, AR42J cells treated with 10M dexamethasone during 48 h. An increase in the number of ZG (arrowhead) and in the cytoplasmic volume can be observed (times 9900). RER, rough endoplasmic reticulum).



Effect of Glucocorticoids on GGT Activity and GP-2 Protein Level in Vivo and in Vitro

In adrenalectomized rats, the pancreatic GGT activity (102 ± 21 milliunits/mg protein) is decreased by about 50% as compared with sham-operated animals (210 ± 35 milliunits/mg protein). Administration of dexamethasone results in a significant (p < 0.001) recovery of the GGT activity (142 ± 25 milliunits/mg protein), whereas an estradiol replacement therapy is without effect on GGT activity (93 ± 20 milliunits/mg protein) that remains at the level found in adrenalectomized animals. The influence of glucocorticoids on GGT activity was also measured in vitro in the pancreatic adenocarcinoma AR42J cells. Incubation of these cells for 24 h, in the presence of 10, 10, and 10M dexamethasone, enhances the GGT activity from 5 milliunits/mg protein (basal level) to 12, 17, and 17 milliunits/mg protein, respectively; this indicates that the dexamethasone effect is maximal at 10M. Culture of AR42J cells at 10M dexamethasone for different periods of time up to 72 h reveals that, after a latent period of 12 h, the GGT activity increases sharply reaching a value that represents 20 times the basal level after a 3-day treatment (Fig. 3). In experiments where the anti-glucocorticoid RU-38486 was added to the culture medium, the increase in GGT activity was minimal (4 milliunits/mg protein) as compared with the basal level (2 milliunits/mg protein). Treatment with estradiol was without effect on GGT activity (data not shown). These in vivo and in vitro data show that GGT activity in the pancreas acinar cells is under the control of glucocorticoids. The higher amplitude of the GGT regulation observed in AR42J cells as compared with the pancreas in vivo might be explained by differences in the hormone concentration in contact with pancreatic cells. In vitro, AR42J cells were treated with 10M dexamethasone, a concentration that induces granulation of these cells as well as maximal induction of GGT activity. The glucocorticoid concentration achieved in the pancreas in vivo during the hormonal therapy might be lower.


Figure 3: Effect of dexamethasone on GGT activity in AR42J cells. Cells in exponential phase of growth were cultured with or without dexamethasone (100 nM) for different periods of time, up to 72 h. GGT activities were obtained from two independent experiments where the assays were carried out in duplicate. Open squares, control cells; solid circles, dexamethasone-treated cells.



GP-2 protein level was measured by the Western blot technique on protein extracts prepared from pancreas and AR42J cells. The general pattern of the proteins appears to be similar among the different samples (Fig. 4). Immunoblotting with GP-2 polyclonal antibodies reveals a single band in control pancreatic extracts. This band exhibits an apparent molecular weight of 78,000 that corresponds to the glycosylated GP2. This polypeptide cannot be detected in the pancreas of adrenalectomized animals, but it reappears following a glucocorticoid replacement therapy (Fig. 4). No GP-2 polypeptide can be detected in AR42J protein extracts even when granule formation has been stimulated by glucocorticoids (Fig. 4).


Figure 4: Western blot analysis of GP-2 protein in rat pancreas and AR42J cells. Left panel, Coomassie Blue staining of protein extracts that are PANCREAS, CONTROL (sham-operated rats), ADX (adrenalectomized rats), ADX + DEX (adrenalectomized rats + dexamethasone), and AR42J, DEX (10M), DEX (10M) (cells treated by 10 and 100 µM dexamethasone during 48 h), CONTROL (cells cultured in absence of dexamethasone). Right panel, detection of GP-2 protein on the Western blot using rabbit GP-2 antibodies. Molecular mass standards (Bio-Rad Labs, Mississauga, Ontario, Canada) are 97.4, 66.4, 45.0, 31.0, 21.5, 14.4 kDa.



Effects of Glucocorticoids on the GGT and GP-2 mRNA Levels in Vivo and in Vitro

Northern blot analysis of pancreatic mRNA prepared from animals with different glucocorticoid status was carried out with the cRNA probe 139A that recognizes all the different GGT mRNA species(20) . Hybridization of this probe to the poly (A) RNA from sham-operated animals (Fig. 5A) reveals a major band which co-migrates with the 2.4-kb GGT band detected in the fetal liver. The 2.4-kb GGT band almost completely disappears in samples from adrenalectomized rats. Administration of dexamethasone to adrenalectomized animals not only prevents the disappearance of this GGT band but also increases its intensity as compared with controls. In contrast, the estradiol replacement therapy does not significantly affect the GGT mRNA level in the pancreas of adrenalectomized rats. A second hybridization of these mRNA samples with an actin probe shows comparable mRNA loading in the four pancreas samples (Fig. 5B). The mRNA samples were further analyzed by hybridization to the cRNA-3 probe specific for the 5`-untranslated sequence unique to the GGT mRNA III (Fig. 5C). This hybridization firmly identifies the 2.4-kb band as the GGT mRNA III previously found in fetal liver and lactating mammary gland(22) . The mRNA III accumulation is under a positive glucocorticoid control since the effect of adrenalectomy is largely compensated by a dexamethasone therapy, whereas estradiol exhibits only a slight effect. The band corresponding to a low molecular weight poly(A) RNA revealed by the cRNA-3 probe in the fetal liver sample (Fig. 5C) has been observed in earlier studies(22) . This 1.6-kb poly(A) RNA is not detected by the GGT probe 139A corresponding to the GGT coding sequence, and the length of this message is shorter than the GGT reading frame. Therefore, this message cannot encode a GGT polypeptide. The interpretation is that a piece of sequence in the GGT mRNA III-specific 5`-untranslated region, used as the probe, may be highly homologous to a sequence present in an unidentified RNA species expressed in the fetal liver. A second GGT band was also observed in pancreas samples from sham-operated animals (Fig. 5A). This band corresponds to a GGT mRNA species that migrates in the gel at a slightly higher rate than the GGT mRNA III. Hybridization to the cRNA-12 probe identifies this mRNA as the GGT mRNA II species that migrates at 2.2 kb (19) (Fig. 5D). It is not expressed in the pancreas of adrenalectomized animals and is not restored by glucocorticoid replacement therapy.


Figure 5: Northern blot analysis of rat GGT mRNA in rat pancreas and AR42J cells. Poly(A) RNA (5 µg) were separated on an agarose denaturing gel and blotted onto a nylon membrane. The blots were hybridized to the GGT cRNA-139A probe that hybridizes to the coding region (A), to the actin cDNA probe (B), to the GGT cRNA-3, a specific probe for the GGT mRNA III (C), and to the GGT cRNA-12, a specific probe for the mRNA II (D). Autoradiography was performed with two intensifying screens at -80 °C for three days. The samples were obtained from fetal liver (FETAL LIVER), from AR42J cells cultured in the absence (-DEX), or in the presence of 100 nM dexamethasone (+DEX) during 48 h and from pancreas from rats with different glucocorticoid status. SHAM, sham-operated; ADX, adrenalectomized; ADX + DEX, adrenalectomized + dexamethasone; ADX + EST, adrenalectomized + estradiol.



To determine whether the GGT mRNA III accumulation in pancreatic cells was under a direct control by glucocorticoids, GGT mRNA accumulation was measured in the AR42J cells. When cultured in the absence of hormone, these cells express the 2.4-kb GGT mRNA at a low level, as revealed by the hybridization to the cRNA-139A probe (Fig. 5A). Addition of 100 nM dexamethasone to the culture medium for 2 days induces a strong increase in the expression of this mRNA species (Fig. 5A), identified as the GGT mRNA III species by hybridization to the cRNA-3 probe (Fig. 5C). Hybridization to the cRNA-12 probe does not reveal any clear signal in AR42J cells (Fig. 5D). Control hybridization to an actin probe shows that equal amounts of RNA were loaded on both lanes (Fig. 5B). Northern blot analysis clearly shows that the increase in the GGT enzyme activity induced by glucocorticoids in pancreatic cells results from the accumulation of the GGT mRNA III.

GP-2 mRNA expression was analyzed in AR42J cells, pancreas, and in other rat tissues. A strong signal corresponding to the 1.9-kb GP-2 mRNA (10) is obtained in the pancreas from sham-operated rats (Fig. 6A). This signal is markedly decreased in the adrenalectomized group, whereas treatment with dexamethasone increases the GP-2 mRNA to a level that is higher than in the control group. Replacement therapy with estradiol also prevents a decrease of GP-2 mRNA level in adrenalectomized rats. A control hybridization with the actin probe (Fig. 6B) does not reveal inequal mRNA loading. No GP-2 mRNA sequences are detected in samples from fetal liver (Fig. 6A) or in adult liver, lactating mammary gland, small intestine, and kidney (data not shown). In AR42J cells, the basal level of GP-2 mRNA is low and does not change significantly following a 48-h treatment by 100 nM dexamethasone (Fig. 6A). It can be noticed that in the dexamethasone-treated sample, the GP-2 mRNA migrates slightly faster than in the control sample, whereas actin mRNA migrate at the same rate in both samples (Fig. 5B). There is no clear explanation for these data; it can only be speculated that both GP-2 mRNA could derive from different transcripts, initiated at different sites on the GP-2 gene, or from the same primary transcript, by alternate splicing or use of different polyadenylation sites.


Figure 6: Northern blot analysis of GP2 mRNA in rat pancreas and AR42J cells. Poly(A) RNA (5 µg) were separated on an agarose denaturing gel and blotted onto a nylon membrane. The blots were hybridized to the GP-2 cRNA probe (A) or to the actin cDNA probe (B). Autoradiography was performed with two intensifying screens at -80 °C for 3 days except the fetal liver and pancreas samples in A (5 h). The samples were obtained from fetal liver (FETAL LIVER), from AR42J cells cultured in the absence (-DEX), or in the presence (+DEX) of 100 nM dexamethasone during 48 h and from pancreas from rats with different glucocorticoid status. SHAM, sham-operated; ADX, adrenalectomized; ADX + DEX, adrenalectomized + dexamethasone; ADX + EST, adrenalectomized + estradiol.



Effect of Glucocorticoids on the Transcription Rates from the GGT Promoter III and GP-2 Promoter

Transcription rates of the GGT mRNA III and GP-2 mRNA were assessed by measuring their transcripts initiated in vivo in a run-on assay, using nuclei isolated from AR42J cells. In control cells, we do not detect any GP-2 transcription signal, whereas GGT transcription signal, clearly above the background, reveals that the GGT promoter III is transcribed at a lower rate than the amylase promoter (Fig. 7, A and B). Treatment of the cells with dexamethasone for 12 or 48 h strongly increases the amylase gene transcription without affecting the GGT promoter transcription rate (Fig. 7).


Figure 7: Dexamethasone effects on GP-2 and GGT gene transcription. AR42J cells were pretreated with 100 nM dexamethasone for 0, 12, or 48 h; nuclei were isolated and allowed to continue transcription in the presence of [alpha-P]UTP. The newly transcribed labeled RNAs were hybridized to a nylon membrane where a GP-2-specific cDNA sequence, pGEM (negative control), the 470-bp GGT genomic sequence described under ``Experimental Procedures,'' and an amylase-specific cDNA sequence have been immobilized. A, autoradiograms were exposed with two intensifying screens at -80 °C for 10 h. B, densitometric analysis of the autoradiogram.



Effects of Glucocorticoids on the GGT mRNA III Degradation

To determine whether glucocorticoids exert their regulatory action at a post-transcriptional level through a stabilization of the GGT transcripts, mRNA III stability was assessed by measuring the decay in GGT mRNA accumulation following an actinomycin D treatment of AR42J cells (Fig. 8). As shown in a representative experiment (Fig. 8A), in control cells a marked and rapid decrease in the GGT mRNA III level occurs a few hours after transcription arrest. A densitometric analysis of this autoradiogram revealed that 82% of the GGT mRNA had disappeared within 2 h (data not shown). In contrast, following a 48-h dexamethasone treatment, the GGT mRNA III level is not significantly affected 4 h after actinomycin D treatment. Analysis of the GGT mRNA III decay curves, obtained by densitometric quantification of the signals on autoradiograms from 6 experiments (Fig. 8B), reveals a much faster degradation rate in untreated as compared with glucocorticoid-treated cells. In the absence of glucocorticoids, the GGT mRNA III decay curve shows a sharp decrease, since 82% of the mRNA transcripts had disappeared within 8 h. In contrast, the GGT mRNA III level decreases by only 34% in dexamethasone-treated cells (Fig. 8B). These results clearly show that glucocorticoids increase the GGT mRNA III level in pancreatic cells by preventing its rapid degradation.


Figure 8: Decay of GGT mRNA III accumulation in AR42J cells treated with actinomycin D. Cells were cultured for 48 h with or without 100 nM dexamethasone prior to the addition of actinomycin D (time 0) at the concentration of 1.25 µg/ml and maintained in culture for up to 8 h. The amount of GGT mRNA III was assessed by an RNase protection assay, using 10-30 µg of RNA extracted from dexamethasone-treated cells and 30-40 µg of RNA extracted from control cells, after different times of treatment with actinomycin D. A, autoradiograms of the GGT-protected sequences obtained from a typical experiment (30 µg RNA) and separated on an acrylamide gel. The undigested probe (362 nucleotides) was loaded on the gel along with the dexamethasone-treated samples. The length of the protected cRNA probe fragment was 294 bases. Autoradiograms were exposed with two intensifying screens, at -80 °C, for 4 days (samples from control cells) and without screen for 24 h (samples from dexamethasone-treated cells). B, GGT mRNA III decay curves. Curves were drawn from average values obtained from three to six independent experiments (± S.E.). For each condition (+ DEX or -DEX), the mRNA accumulation remaining after different times of exposure to actinomycin D is expressed as a percentage of the mRNA level before the addition of the drug (time 0: 100%) and plotted against time on a semi-logarithmic scale. Open triangles, dexamethasone-treated cells; solid circles, control cells.




DISCUSSION

To gain insight into the mechanisms of ZG formation in pancreatic acinar cells, we investigated the influence of glucocorticoids and estradiol on the expression of GGT and GP-2 proteins in the rat pancreas in vivo and in vitro, using the AR42J pancreatic carcinoma cell line. Adrenalectomy caused a marked depletion of zymogen granules that was prevented by glucocorticoid replacement therapy (Fig. 1) as described previously(4) . In adrenalectomized animals we observed a decrease in the GP-2 mRNA level that cannot be related to a specific effect of glucocorticoids since it can also be prevented by estradiol (Fig. 6). The amount of GP-2 protein in pancreas is correlated to the GP-2 mRNA level under different glucocorticoid status (Fig. 4). In AR42J cells, however, glucocorticoid treatment, which promotes extensive granulation of these cells (Fig. 2), induces neither the GP-2 mRNA nor the GP-2 protein level ( Fig. 4and Fig. 6). These data show that granule formation can occur independently of GP-2 synthesis. This fact is corroborated by the absence of GP-2 mRNA in the lactating mammary gland (data not shown), an organ very active in protein secretion. In a recent study, Dittié and Kern (34) reached similar conclusions based on the following observations. 1) GP-2 mRNA was undetectable in fetal pancreas during the differentiation period, including when ZG formation takes place. 2) GP-2 mRNA synthesis does not occur in parotid and adrenal glands. 3) Glucocorticoids are without effect on GP-2 mRNA accumulation in AR42J cells.

In contrast to GP-2, GGT expression is clearly under a direct positive control of glucocorticoids. This is supported by a decrease of both enzyme activity and mRNA level in adrenalectomized animals and by prevention of these effects with dexamethasone but not with an estradiol replacement therapy (Fig. 5). This direct effect of the hormone can be confirmed in vitro in AR42J cells that respond to dexamethasone by a marked increase in the GGT activity (Fig. 3). Northern blot analysis clearly showed that the increase in mRNA induced by glucocorticoids, observed both in vivo and in vitro, results from an accumulation of the GGT mRNA III (Fig. 5), transcribed from GGT promoter III on the GGT gene(22) . The induction of the GGT expression by glucocorticoids is not due to a direct effect of the hormone receptor complex onto the palindromic target sequence, previously identified on the GGT promoter III(22) , or to the participation of glucocorticoid-regulated factors that could act at the level of the GGT gene. In fact, no hormonal effect can be observed on the transcription rate of the GGT promoter III in AR42J cells after a 48-h glucocorticoid exposure (Fig. 7), conditions which induce markedly the GGT mRNA III accumulation. Under the same conditions, we observed an increase in the amylase gene transcription rate that is known to be mediated by a glucocorticoid-induced factor (35) . In contrast, our data show that the glucocorticoid treatment has a strong stabilizing effect on the GGT mRNA III by preventing the rapid decay observed in control cells (Fig. 8). The effect of glucocorticoids on GGT activity is prevented by the anti-glucocorticoid RU-38486. This indicates that the effect requires binding of the hormone to its receptor and subsequent interaction of this complex with a glucocorticoid-responsive gene encoding a protein that is able to modulate the GGT transcript degradation rate. This effect on mRNA stability, which would require RNA and protein synthesis, is most consistent with the long lag observed between addition of the hormone and induction of GGT activity. Such a post-transcriptional effect of the glucocorticoids on mRNA half-life has already been reported for insulin(36) , growth hormone, and its receptor(37) . The mechanisms of this regulation are not yet clearly known, but the presence in these mRNAs of unique sequences that could act as a target for glucocorticoids stabilizing or destabilizing factors has been proposed.

In contrast to GP-2, GGT synthesis parallels the zymogen granule content in pancreatic cells in vivo and in vitro in AR42J cells. During development, patterns of GGT and amylase expression are biphasic and comparable(38) . This developmental profile corresponds to the massive granule formation that occurs before birth and at the weaning period (39) and has been associated to the fluctuating levels of glucocorticoids(40) . All these data support the view that GGT protein expression is associated with zymogen granule formation. The quantitative differences observed between the extent of granulation and GGT activity in the pancreas from adrenalectomized rats subjected to glucocorticoid therapy indicate that a partial recovery of GGT activity might be sufficient to obtain optimal granulation. However, the precise roles for GGT and its substrate, glutathione (GSH), in the secretory process are still conjectural. Glutathione is the major redox buffer in the cell, and its role in protein secretion has been emphasized(41) . Moreover, it has been shown that the GHS/GSSG ratio, which exhibits a value greater than 30 in the cytoplasm, drops to nearly 5 in the secretory pathway(16) , a ratio suitable for an optimal oxidative protein folding catalyzed by a disulfide isomerase (42) . The mechanism maintaining this low GSH/GSSG ratio remains elusive. We speculate that GGT, by initiating GSH degradation into cysteinyl glycine in the granule, may contribute to keeping it in a more oxidized state, since cysteinyl glycine can easily undergo a rapid nonenzymatic oxidation(43, 44) .

In conclusion, this study shows that ZG formation induced by glucocorticoids is closely linked to GGT expression. The localization of this enzyme in the granules of the pancreas and other secretory glands(8) , as well as its induction in the lactating mammary gland (45) , suggests that glucocorticoids may play a significant role in the packaging process by regulating the expression of GGT in these glands. The glucocorticoids appear now to have a well integrated function interacting at different levels of the secretory process, synthesis of secretory proteins as reported for amylase (35) or casein(46) , increase in the number of cholecystokinin receptors(47) , and also synthesis of protein components of secretory vesicles, as demonstrated in this study.


FOOTNOTES

*
This work was supported by the Institut National de la Santé et de la Recherche médicale (France), by the Natural Science and Engineering Research Council (NSERC) (Canada), the Government of Quebec Fond pour la Formation de Chercheurs et Aide à la Recherche (FCAR), and by a grant from the cooperation Franco-Québecoise en Recherche médicale. The costs of publication of this article were defrayed in part by the payment of page charges. This article must therefore by hereby marked ``advertisement'' in accordance with 18 U.S.C. Section 1734 solely to indicate this fact.

§
To whom correspondence should be addressed: INSERM Unité 99, Hôpital Henri Mondor, 94010 Créteil, France. Tel.:(33) -1 49 81 35 44; Fax:(33) -1 48 98 09 08; Laperche{at}infobiogen.fr.

(^1)
The abbreviations used are: ZG, zymogen granule; GP-2, glycoprotein 2; GGT, -glutamyl transpeptidase; PBS, phosphate-buffered saline; kb, kilobase; bp, base pair(s); GSH, glutathione; GSSG, glutathione disulfide.


ACKNOWLEDGEMENTS

We wish to thank Dr. M. J. Rindler and R. J. MacDonald for the generous gifts of the GP-2 and amylase cDNA recombinant plasmids and Dr. T. Rohn for the careful correction of this manuscript.


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