Identification of Early Growth Response Gene-1 (Egr-1) as a Phorbol Myristate Acetate-induced Gene in Lung Cancer Cells by Differential mRNA Display

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Identification of Early Growth Response Gene-1 (Egr-1) as a Phorbol Myristate Acetate-induced Gene in Lung Cancer Cells by Differential mRNA Display

Liang You and Sonia B. Jakowlew

National Cancer Institute, Medicine Branch, Rockville, Maryland

Abstract

Top
Abstract
Introduction
Materials & Methods
Results
Discussion
References

Cellular regulatory genes including transcription factors may play an important role in the induction, maintenance, and progressionof lung cancer. These regulatory genes are inducible by variousmitogenic stimuli including phorbol myristate acetate (PMA). Thedifferential mRNA display method was used to identify potentialearly response genes regulated by PMA in non-small cell lung cancer(NSCLC) cell lines. Using this technique, several cDNA fragmentswere found to be potentially differentially regulated by PMA inthe squamous NSCLC cell line NCI-H157. One of these cDNA fragmentsof approximately 100 bp was determined to be differentially inducedby at least 30-fold by PMA by northern blot analysis and to hybridizeto a single 3.4 kb mRNA species. This cDNA fragment was cloned,sequenced, and identified to be identical to a portion of the3'-untranslated region of the human early growth response gene-1(Egr-1). Using Egr-1 cDNA as a probe, it was demonstrated thatPMA induces Egr-1 mRNA expression in at least three other NSCLCcells as well. In addition, PMA caused a transient increase inexpression of the Egr-1 transcript reaching a maximum level by1 h before decreasing in NCI-H157 and three other types of NSCLCcells. Treatment of these NSCLC cells with TGF- $beta$ ₁ showed a transientincrease in Egr-1 mRNA similar to PMA which also reached a maximumlevel after 1 h. Normal human bronchial epithelial (NHBE) cellsalso showed a rapid, transient increase in expression of Egr-1mRNA after treatment with PMA. In contrast, treatment of NHBEcells with TGF- $beta$ ₁ showed that expression of Egr-1 mRNA increasedby 1 h but reached a maximum level only after 6 h. These resultsindicate that both PMA and TGF- $beta$ ₁ can induce Egr-1 mRNA expressionin NSCLC cells and NHBE cells; however, while PMA induces Egr-1mRNA similarly in both cell types, TGF- $beta$ ₁ induces Egr-1 mRNA expressionmore rapidly and more transiently in NSCLC cells than in NHBEcells. Our results suggest that Egr-1 may play different rolesin response to mitogens in normal and malignant lung cells.

	Introduction

Top Abstract Introduction Materials & Methods Results Discussion References

Lung cancer is the leading cause of cancer death in both men and women, accounting for 30% of all cancer-related mortalityin the United States (1). Even though some improvement hasbeen made in clinical management of lung cancer, the current 5-yrsurvival rate is only about 13% (2). The diagnosis of lungcancer is usually too late and current therapeutic strategiesare inadequate. Lung cancer, especially non-small cell lung cancer(NSCLC), remains refractory to all available systematic treatmentoptions (3). Any major impact in the prevention and/or treatmentof this disease is largely dependent upon a better understandingof the molecular aspects of the pathogenesis of lung cancer.

Proto-oncogenes and tumor suppressor genes are cellular genes that regulate other genes involved in the control of normalcellular growth and differentiation. These genes code for growthfactors, growth factor receptors, kinases which phosphorylatediverse cellular substrates, and DNA binding proteins which regulateexpression of numerous cellular genes. Oncogenesis may occur throughactivation of dominant growth promoting proto-oncogenes (suchas Her-2/neu, ras, and myc) where mutation or overexpression ofthe gene product induces malignancy, and inactivation of growthinhibitory tumor suppressor genes (such as p53 and Rb) where theabsence of expression or function of these genes results in malignancy,or both (4, 5). Defects in pathways controlling growth anddifferentiation can effect the development of malignancy includinglung cancer.

One approach to identifying genes that may play key roles in cellular growth control is to focus on transcripts whose expressionis low in nondividing cells but is rapidly increased when stimulatedby mitogens. Immediate early genes are among the earliest downstreamnuclear targets for ligand-receptor interactions. These genesare induced in the absence of de novo protein synthesis and wereinitially identified as promoters of cell proliferation becausetheir expression is required for quiescent cells to enter thecell-cycle. The best characterized immediate early genes are c-junand c-fos (6, 7); both genes encode transcription factorsthat bind to specific regulatory sequences and activate expressionof responsive genes. c-jun has a leucine zipper motif, which formsa heterodimer with a variety of proteins including c-fos. Thejun-fos protein complex, also known as AP-1, binds to a numberof cellular promoters through a common element (5'-TGACTCA-3').At present, it is thought that these genes have bifunctional activitybecause they appear to be able to both activate and repress transcriptionof responsive genes.

Phorbol myristate acetate (PMA), a tumor-promoting phorbol ester, is a potent mitogen that can activate gene expression ofa number of genes, including immediate early genes like jun andfos. Recently, it has been reported that PMA can enhance the growthinhibitory activity of negative growth factors like transforminggrowth factor- $beta$ (TGF- $beta$ ) in human prostate cancer cell lines (8).PMA has also been shown to increase the steady-state level ofTGF- $beta$ ₁ mRNA in different cell types. In addition, it has alsobeen shown that both PMA and TGF- $beta$ ₁ can inhibit mitogenesis througha similar signal transduction pathway involving protein kinaseC (PKC) in both mesengial and vascular smooth muscle cells (9).

The differential mRNA display method, originally introduced by Liang and Pardee in 1992 (10), has been succesfully usedto isolate genes differentially expressed between normal and cancercells, and between cells cultured in the presence and absenceof growth factors and chemical agents (11). In this method,only a small amount of RNA is required from two different populationsof cells that is reverse-transcribed using anchored oligo-dT primersand random 5' oligonucleotide primers. The patterns of amplifiedcDNA fragments are displayed side-by-side on a polyacrylamidegel, individual bands that indicate differential expression arerecovered, reamplified, subcloned, and sequenced. The result istypically a 50-500 bp cDNA sequence which may correspond to the3' end of a cDNA of a known gene obtained from available DNA databases.

In this study, differential mRNA display was used to identify PMA-regulated immediate early genes in NSCLC cells and normalhuman bronchial epithelial (NHBE) cells. One of these genes wasidentified to be early growth response gene-1 (Egr-1). Egr-1 mRNAexpression was found to be regulated similarly by PMA in bothNSCLC cells and NHBE cells reaching a maximum level by 1 h beforedecreasing; in contrast, it was shown that Egr-1 mRNA was differentiallyregulated by TGF- $beta$ ₁ in these different cell types. Our resultssuggest that Egr-1 may play different roles in response to mitogensin normal and malignant lung cells.

	Materials and Methods

Top Abstract Introduction Materials & Methods Results Discussion References

Cell Culture and RNA Isolation

Human lung cancer NSCLC cell lines (NCI-H157, -H226, -H727, -H838, -H1264, -H1299, and -H2170) were cultured in serum-supplementedmedium at 37°C [RPMI-1640 medium (GIBCO/BRL, Grand Island, NY)]containing 10% heat-inactivated fetal bovine serum (GIBCO/BRL)(12, 13). NHBE cells obtained from Clonetics (San Diego, CA)were cultured in bronchial epithelial growth medium supplied withthe cells. Then NSCLC cells were split weekly by using trypsin/EDTA(GIBCO/BRL, Rockville, MD). Routinely, the cells showed greaterthan 90% viability, were Mycoplasma free, and were used when theywere in exponential growth phase. The NHBE cells were routinelyused without splitting. For treatment of cells with PMA and TGF- $beta$ ₁,cells were washed with phosphate-buffered saline and incubatedwith RPMI-1640 medium containing 0.1% bovine serum albumin (BSA).PMA was obtained from Sigma (St. Louis, MO). Human TGF- $beta$ ₁ wasobtained from R&D Systems (Minneapolis, MN). Total RNA was isolatedfrom NSCLC and NHBE cells by the method of Chirgwin and associates(14), and was treated with RNase-free DNase (GIBCO/BRL).

Differential mRNA Display

Purified total cell RNA (0.2 µg) was reverse transcribed in a 20-ul reaction mixture with Superscript reverse transcriptase(GIBCO/BRL) and oligo-dT primer T₁₁C at 37°C for 60 min. For PCRamplification, 2 µl of reverse transcribed sample was mixed with18 µl of mixture containing the oligo-dT primer T₁₁C and a randomprimer 5'-AAGCTTGATTGCC-3' (AP-1). Radioactive [³³P]- $alpha$ -dATP was added in the PCR reaction and the reaction mixturewas subjected to 40 cycles of PCR using parameters of 94°C for30 s, 40°C for 2 min, and 72°C for 30 s according to the RNAimagekit (GenHunter Co., Nashville, TN). Radiolabeled PCR productswere analyzed by electrophoresis on 6% polyacrylamide gels. Thegels were dried and then exposed to Kodak XAR-5 film (Kodak Co.,Rochester, NY).

Reamplification of cDNA Fragments

Differentially expressed cDNA fragments were identified and recovered from the gel and reamplified in a 40-cycle PCR usingthe same pair of primers described previously, T₁₁C and AP-1 (GenHunterCo.). Reamplified cDNA fragments were separated by electrophoresison a low-melting agarose gel, extracted using the GENECLEAN IIKIT (BIO 101, Vista, CA) and the purified cDNA fragments wereused as templates for random priming and for TA cloning.

Northern Blot Analysis

Equal amounts of total RNA (10 µg) were electrophoresed on 1% agarose gels containing 0.66 M formaldehyde, transferred to"Nytran" filters (Scleicher and Schuell, Keene, NH), UV-cross-linkedand baked for 3 h. Ethidium bromide (33 µg/ml) was included inboth the gels and running buffers to visualize the positions ofribosomal RNAs by UV illumination after eletrophoresis. Blotswere hybridized with [³²P]-labeled (3,000 Ci/mmol, Dupont, Boston, MA) random-primed cDNAprobes at 65°C according to Church and Gilbert (15), and thenexposed for various times at $-$ 70°C using an intensifying screen.Densitometry of autoradiograms was performed using a scanninglaser densitometer.

cDNA Probes

Hybridization was performed using the following cDNA probes: 1.6 kb XbaI-HindIII fragment of human Egr-1, plasmid pOC68, obtainedfrom V. Sukhatme (16, 17); 1.0 kb EcoRI fragment of humanc-fos, obtained from T. Curran (18); 0.9 kb XbaI-HindIII fragmentof rat TGF- $beta$ ₁, plasmid pRTGF- $beta$ ₁, obtained from S. W. Qian (19).

TA Cloning and Sequencing Analysis

Reamplified cDNA fragments were cloned into the plasmid vector pCRII using the TA cloning kit (Invitrogen, San Diego, CA)and purified by the QIAGEN plasmid kit (QIAGEN, Inc., Chatsworth,CA). The cDNAs were sequenced with T7 and SP6 primers using thedye terminator cycle sequencing core kit and an Applied Biosystemsautomated sequencer (Perkin Elmer, Foster City, CA). The nucleotidesequences obtained were compared with known sequences by searchingthe Genbank and EMBL databases with the BLAST (National Centerfor Biotechnology Information, Bethesda, MD).

	Results

Top Abstract Introduction Materials & Methods Results Discussion References

We have previously shown that PMA is able to induce expression of several genes in lung cancer cells including c-fos and TGF- $beta$ ₁(20, 21). To examine the effect of PMA on expression of potentiallyinducible novel genes in NSCLC cells, exponentially growing subconfluentcultures of human lung squamous carcinoma cells (NCI-H157) weretreated with PMA (1 µM) for different times from 1 h to 24 h inRPMI-1640 medium containing 0.1% BSA. The optimal amount of PMAadded was based on prior studies (20). Total RNA was extractedfrom these cells and northern blot analysis was performed witha radiolabeled random-primed cDNA probe for c-fos. Within 1 hof addition of PMA, there was a transient 15-fold increase inthe level of the 2.2 kb c-fos transcript which decreased by 3h (Figure 1A). To examine expression of TGF- $beta$ ₁, the blot thatwas used to investigate expression of c-fos was dehybridized,exposed to film to ensure complete dehybridization, and then hybridizedwith a cDNA probe for TGF- $beta$ ₁. Within 6 h of addition of PMA, therewas an 8-fold increase in the level of the 2.5 kb TGF- $beta$ ₁ transcriptwhich persisted to 24 h (Figure 1B). To examine the regulationof c-fos and TGF- $beta$ ₁ by PMA in normal lung cells, sub-confluentcultures of NHBE cells were incubated with PMA as described forthe NSCLC cells. Total RNA was extracted from these cells at theindicated times, and northern blot analysis was performed usinga c-fos cDNA probe. Figure 1D shows that the level of expressionof c-fos mRNA increased 12-fold by 1 h in NHBE cells followingtreatment with PMA. When this blot was rehybridized with a cDNAprobe for TGF- $beta$ ₁, the level of TGF- $beta$ ₁ mRNA increased 2.5-foldby 3 h and then an additional 2- and 6-fold by 6 and 24 h, respectively,in these cells (Figure 1E). As a control, the gels were stainedwith ethidium bromide and photographed to ensure that approximatelyequal amounts of RNA had been applied to the gels (Figures 1Cand 1F).

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Figure 1. Northern blot analysis of c-fos and TGF- $beta$ ₁ mRNAs in NCI-H157 and NHBE cells after treatment with PMA. Total RNA (10 µg) wasisolated from exponentially growing subconfluent (panels A andB) NCI-H157 cells and (panels D and E) NHBE cells cultured with1 µM PMA for 0 h (lanes 1, 6), 1 h (lanes 2, 7), 3 h (lanes 3,8), 6 h (lanes 4, 9) and 24 h (lanes 5, 10), separated by electrophoresison a 1% agarose-formaldehyde gel, and transferred to a Nytranfilter as described in MATERIALS AND METHODS. Hybridization wasperformed with (panels A and D) c-fos cDNA probe; (panels B andE) TGF- $beta$ ₁ cDNA probe. The blots were exposed for 1 day. PanelsC and F show the ethidium bromide staining pattern of the gelsshowing 18S and 28S rRNA. The blots shown in this and subsequentfigures are representative of three separate experiments.

Differential mRNA display analysis was used to identify early response genes regulated by PMA in lung cancer cells. For thispurpose, total RNAs were isolated from exponentially growing subconfluentcultures of NCI-H157 raised either in the absence of or presenceof two concentrations of PMA. cDNAs were synthesized by reversetranscriptase and amplified using a one-base anchored oligo-dTprimer (T₁₁C) as described in MATERIALS AND METHODS. Forty cyclesof amplification were performed with an oligo-dT primer (5'-T₁₁C-3')and a random primer (5'-AAGCTTGATTGCC-3'). The amplified radiolabeledcDNA products were size fractionated on denaturing urea-polyacrylamidegels and differentially expressed cDNAs were identified by autoradiography.A representative differential display pattern observed with RNAsisolated from untreated NCI-H157 cells and cells treated withtwo concentrations of PMA is shown in Figure 2A. Several reproduciblebands appeared to represent potential differentially regulatedcDNA fragments (Figure 2A, arrows); while the majority of thesebands showed a strong signal resulting after treatment with PMA,at least two bands showed a strong signal without treatment withPMA. Among the potential differential cDNAs indicated by arrows,one of approximately 100 bp indicated by the thick arrow had thestrongest signal and the most dramatic change (thickness of theband) after PMA treatment. This cDNA fragment was excised fromthe gel and reamplified by another round of PCR using corresponding5' and 3' primers.

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Figure 2. Differential mRNA display analysis of PMA-affected genes. Panel A: Total RNA was isolated from untreated ( $-$ ) (lane 1) or PMAtreated (+) (lane 2, 1 µM PMA; lane 3, 5 µM PMA) cultures of NCI-H157cells and reverse transcribed to cDNA for further mRNA differentialdisplay amplification. The amplified cDNA fragments were separatedby electrophoresis on 6% DNA sequencing gels and autoradiographedas described in MATERIALS AND METHODS. Thin arrows indicate theposition of differentially displayed cDNA bands. The thick arrowindicates the position of the 100 bp PMA-induced cDNA fragment.DNA molecular weight markers are indicated at the right. PanelB: Northern blot analysis of PMA-induced mRNAs in NCI-H157 cells.Total RNA (10 µg) was isolated from exponentially growing subconfluentNCI-H157 NSCLC cells cultured for 1 h with: no addition (lane1); 1 µM PMA (lane 2); 5 µM PMA (lane 3), and analyzed as beforewith (panel B) PMA-induced gene cDNA probe; (panel C) c-fos cDNAprobe. The blots were exposed for 1 day. Panel D: The ethidiumbromide staining pattern of the gel showing 18S and 28S rRNA.

To reconfirm the differential expression pattern of the 100 bp cDNA fragment, the excised reamplified cDNA fragment was usedas a probe to hybridize to northern blots containing total RNAfrom NCI-H157 cells cultured in the presence or absence of PMAfor 1 h. Northern blot analysis demonstrated that this cDNA fragmenthybridized to a transcript of 3.4 kb in NCI-H157 cells after treatmentwith two concentrations of PMA; within 1 h of addition of PMA,there was at least a 30-fold increase in the level of this transcript(Figure 2B). Expression of c-fos mRNA was also examined in thesecells cultured in the presence or absence of PMA. To examine expressionof c-fos, the blot that was used to investigate expression ofthe 3.4 kb mRNA induced by treatment with PMA was dehybridized,exposed to film to ensure complete dehybridization, and then hybridizedwith a cDNA probe for c-fos. Hybridization with a cDNA probe forc-fos showed an increase in expression of c-fos mRNA of at least60-fold after treatment with PMA in NCI-H157 cells (Figure 2C).As a control, the gel was stained with ethidium bromide and photographedto ensure that equal amounts of RNA had been applied to the gel(Figure 2D).

Following northern blot hybridization analysis, the PMA-induced cDNA fragment was subcloned into plasmid DNA and the insertfrom plasmid DNA was also shown to hybridize to the same sizemRNA and exhibit differential expression in PMA-treated NCI-H157cells (data not shown). It was determined that this plasmid DNAfragment has an insert of 88 bp and sequence analysis confirmedthat it contained both 5' (AP-1) and 3' (T₁₁C) primer sequencesused for amplification. After DNA sequence homology searches inGenbank database, the sequence was found to be identical to aportion of the 3'-untranslated region of the cDNA sequence ofthe human early growth response-1 gene (Egr-1) (Figure 3). Onemismatch was observed in the random primer region.

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Figure 3. Nucleotide sequence of PMA-induced gene. Reamplified PMA-induced gene cDNA fragment was cloned into a TA cloning vector andsequenced using SP6 and T7 primers. The sequence was searchedin GenBank data base. Homology of the PMA-induced gene with Egr-1is indicated. The 5'-untranslated, coding and 3'-untranslatedregions of human Egr-1 cDNA are shown.

To determine whether Egr-1 mRNA is also induced by PMA in other squamous NSCLC cell lines, three additional squamous NSCLCcell lines including NCI-H226, NCI-H1264, and NCI-H2170 were culturedin the presence of PMA and analyzed by northern blot hybridization.Figure 4A shows that expression of Egr-1 mRNA increased approximately20-, 40-, and 40-fold in NCI-H226, NCI-1264, and NCI-H2170, respectively,following treatment with PMA. To determine whether Egr-1 mRNAis induced by PMA in other NSCLC cell lines besides the squamoustype, three other NSCLC cell lines representing additional typesof NSCLC were examined including NCI-H727 (carcinoid), NCI-H838(adenocarcinoma) and NCI-H1299 (large cell carcinoma). Exponentiallygrowing subconfluent cultures of these NSCLC cells were treatedwith PMA for different times from 1 h to 24 h in RPMI-1640 mediumcontaining 0.1% BSA. Total RNA was extracted from these cellsat increasing times and northern blot analysis was performed withan Egr-1 cDNA probe. Within 1 h of addition of PMA, there wasan increase in expression of Egr-1 mRNA by 60-, 100-, 30-, and50-fold in NCI-H157, NCI-727, NCI-H838, and NCI-H1299, respectively(Figure 5A); this increase was transient and decreased by 3 hfollowing treatment with PMA. A second increase in Egr-1 mRNAwas observed 6 h following treatment with PMA in NCI-H157 andNCI-H727 before decreasing after 24 h to basal levels; this secondincrease was only about 30% of the level at 1 h in each cell line.No second increase was detected in NCI-H838 or NCI-H1299 followingtreatment with PMA.

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Figure 4. Northern blot analysis of EGR-1 mRNA in squamous NSCLC cells. Panel A: Total RNA (10 µg) was isolated from subconfluent exponentiallygrowing NSCLC cells including NCI-H157, NCI-H226, NCI-H1264 andNCI-H2170 and cultured for 1 h with: no addition ( $-$ ) (lanes 1,3, 5 and 7); 1 µM PMA (+) (lanes 2, 4, 6 and 8). The blots wereexposed for 1 day. Panel B: The ethidium bromide staining patternof the gels showing 18S and 28S rRNA.

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Figure 5. Effect of PMA on expression of Egr-1 mRNA in NSCLC cell lines. Panel A: Total RNA (10 µg) isolated from subconfluent exponentiallygrowing NSCLC cell lines NCI-H157, NCI-H727, NCI-H838, and NCI-H1299cultured with 1 uM PMA for 0 h (lanes 1, 6, 11 and 16), 1 h (lanes2, 7, 12 and 17), 3 h (lanes 3, 8, 13 and 18), 6 h (lanes 4, 9,14 and 19) and 24 h (lanes 5, 10, 15 and 20) and analyzed as beforewith Egr-1 cDNA probe. The blot was exposed for 1 day. Panel B:The ethidium bromide staining pattern of the gel showing 18S and28S rRNA.

In addition to investigating the effect of PMA on expression of Egr-1 mRNA in NSCLC cells, the effect of TGF- $beta$ ₁ on expressionof this transcript was also examined in these cells. Expressionof Egr-1 mRNA increased maximally at levels of 60-, 100-, 15-,and 50-fold in NCI-H157, NCI-727, NCI-H838, and NCI-H1299, respectively,by 1 h following treatment with TGF- $beta$ ₁ (Figure 6A). The Egr-1mRNA expression decreased by 3 h in each cell line with a secondincrease occurring after 6 h in NCI-H727 which persisted for 24h. A minor second increase in Egr-1 mRNA also occurred at 6 hin NCI-H157, and decreased to basal level by 24 h.

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Figure 6. Effect of TGF- $beta$ ₁ on expression of Egr-1 mRNA in NSCLC cell lines. Panel A: Total RNA (10 µg) was isolated from subconfluentexponentially growing NSCLC cell lines cultured with 5 ng/ml TGF- $beta$ ₁for 0 h (lanes 1, 6, 11 and 16), 1 h (lanes 2, 7, 12 and 17),3 h (lanes 3, 8, 13 and 18), 6 h (lanes 4, 9, 14 and 19) and 24h (lanes 5, 10, 15 and 20) and analyzed as before with Egr-1 cDNA.The blot was exposed for 1 day. Panel B: The ethidium bromidestaining pattern of the gel showing 18S and 28S rRNA.

In addition to investigating the effect of PMA and TGF- $beta$ ₁ on expression of Egr-1 mRNA in NSCLC cells, the effect of theseagents on expression of Egr-1 mRNA was also examined in NHBE cells.Figure 7A shows that Egr-1 mRNA was induced maximally (20-fold)at 1 h after PMA treatment before decreasing to 50% of this levelby 3 h and to basal level by 24 h. Following treatment with TGF- $beta$ ₁,expression of Egr-1 mRNA increased 2-fold by 1 h and reached amaximal level only after 6 h where expression was 10-fold higherthan at the initial time (Figure 7B); expression of Egr-1 mRNAdecreased to basal levels by 24 h following treatment with TGF- $beta$ ₁in NHBE cells.

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Figure 7. Effect of PMA and TGF- $beta$ ₁ on expression of Egr-1 mRNA in NHBE cells. Total RNA (10 µg) was isolated from subconfluent NHBEcells cultured with panel A: 1 µM PMA; panel B: 5 ng/ml TGF- $beta$ ₁for 0 h (lane 1); 1 h (lane 2); 3 h (lane 3); 6 h (lane 4); 24h (lane 5). The blots were exposed for 2 days. The ethidium bromidestaining pattern showing 18S and 28S rRNA is shown below eachblot.

	Discussion

Top Abstract Introduction Materials & Methods Results Discussion References

Regulation of cellular growth and proliferation is dependent on a number of gene families including growth factors, growthfactor receptors, proto-oncogenes, and transcription factor genes.It has been suggested that some transcription factors play a rolein the regulation of normal lung physiology. In the present study,differential mRNA display was used to identify Egr-1 as a generegulated by PMA in NSCLC cells. In addition, we have shown thatexpression of Egr-1 mRNA is also regulated by PMA in NHBE cells.The biochemical processes that precede immediate early gene inductionafter mitogenic stimulation include signal transduction throughprotein kinase activation. PKC is the cellular receptor for phorbolesters like PMA that can initially activate some PKC isoenzymesand then downregulate them (22, 23). Since PMA has been shownto elicit both growth promotion and growth inhibition in differentcells and both higher and lower levels of PKC have been foundin cancer cells as compared to normal cells, it has been suggestedthat PKC may participate in negative feedback of growth. Althoughthe expression of Egr-1 has been most commonly observed aftertreatment with mitogenic stimuli, a consistent requirement forprogression through the cell cycle has not been observed, leavingthe role of Egr-1 in control of cell proliferation unclear. Immediateearly response genes were initially identified as promoters ofcell proliferation because their expression was thought to berequired for quiescent cells to enter the cell cycle (24). However,because some of these genes like fos have been shown to be induciblethroughout almost all stages of the cell cycle, activation ofsome of these genes may not be limited to the mitogenic response.Our study shows that Egr-1 mRNA is rapidly induced by PMA in NSCLCand NHBE cells. While maximal expression of Egr-1 mRNA was detectedwithin 1 h following treatment with PMA, a second increase inexpression of this mRNA, although smaller than the first, wasdetected by 6 h in some of these cells. This secondary increasein Egr-1 mRNA may indicate the induction of other genes whichalso act to regulate Egr-1. Also, while PMA was shown to rapidlyregulate Egr-1 mRNA in NSCLC cells, it remains to be determinedwhether the Egr-1 protein is also rapidly translated and regulatedin these different lung cell types.

In addition to regulation by PMA, it was also demonstrated in the present study that Egr-1 mRNA is rapidly induced by TGF- $beta$ ₁in NSCLC cells as well. We have shown in a recent study expressionof the mRNAs and proteins for the different TGF- $beta$ ligands andreceptors in NSCLC cells (25). Egr-1 is a member of a zinc-fingergene family consisting of at least four transcription factors(Egr-1, -2, -3, and -4) that preferentially binds GC-rich regulatoryelements (GCEs) with the sequence 5'-GCGT/GGGGCG-3'or 5'-TCCT/ACCTCCTCC-3'(26). The promoter of the human TGF- $beta$ ₁ gene has been shown tocontain multiple GC-rich sequences (27). The expression of TGF- $beta$ ₁is regulated in part by these GC-rich sequences (27, 28).Wilms tumor-1 protein (WT1) is a strong repressor of the transcriptionalactivity of the human TGF- $beta$ ₁ promoter whose effect is counteractedin a dose-dependent manner by coexpression of Egr-1 (29). Recently,it has been shown that expression of Egr-1 in human HT-1080 fibrosarcomacells causes increased secretion of biologically active TGF- $beta$ ₁in direct proportion to the amount of Egr-1 expressed (30);addition of exogenous TGF- $beta$ ₁ to Egr-1-expressing HT1080 cellsinhibits their growth and addition of monoclonal anti-TGF- $beta$ ₁ antibodiesto these cells completely reverses the growth inhibitory effectsof Egr-1. The more persistent increase in Egr-1 mRNA in responseto TGF- $beta$ ₁ in NHBE cells compared to NSCLC cells may act to feedbackand increase the level of TGF- $beta$ ₁ and thus inhibit the proliferationof these cells. It remains to be determined whether the persistentincrease in Egr-1 mRNA in NHBE cells also occurs at the proteinlevel to enable this to occur.

The effects of PMA and TGF- $beta$ ₁ have been examined previously in normal and neoplastic human bronchial epithelial cells. Differentialeffects of PMA and TGF- $beta$ ₁ have been demonstrated in these differenthuman bronchial epithelial cells. For example, while as littleas 3 nM PMA was shown to induce NHBE cells to undergo terminaldifferentiation and completely inhibit their proliferation, thegrowth of several NSCLC cell lines was not significantly inhibitedat this concentration NSCLC cells and continued to proliferatein as much as 100 nM PMA (31). While NHBE cells and severalNSCLC cell lines possess comparable numbers of TGF- $beta$ receptorswith similar affinities, TGF- $beta$ ₁ has been shown to inhibit DNAsynthesis, proliferation and differentiation of NHBE cells, butnot to inhibit these activities in NSCLC cells (32). Lung cancercells apparently acquire differentiation-resistent phenotypesat a step of the differentiation-induction pathway other thanat the ligand binding of the surface receptors for the differentiationinducers. We have demonstrated a transient increase in Egr-1 mRNAin NSCLC cells following exposure to either PMA or TGF- $beta$ ₁. Whilethe effect of PMA on Egr-1 mRNA is also transient in NHBE cells,the effect of TGF- $beta$ ₁ on Egr-1 mRNA is more prolonged in thesecells. Cell density has been shown to govern the ability of TGF- $beta$ ₁to control differentiation in NHBE cells. For example, it hasbeen demonstrated that whereas irreversible inhibition of DNAsynthesis occurs in sparse cell density cultures of NHBE cellswithin 24 h after exposure to TGF- $beta$ ₁, only a transient depressionin DNA synthesis is seen in high density cultures (33). Recently,we have demonstrated the ability of TGF- $beta$ ₁ to inhibit the proliferationof some NSCLC cells in soft agarose (25). It is possible thatcell density has a role in controlling the ability of TGF- $beta$ ₁ toinhibit proliferation of lung cancer cells just as it does inNHBE cells. It is also possible that cell density may have aneffect on the regulation of Egr-1 in these cells. Additional studieswill be needed to determine whether this is the case.

Since Egr-1 is a positive regulator of TGF- $beta$ ₁, it may be important that Egr-1 is low or undetectable in most human tumorsthat have been investigated. For example, in a series of 101 pairedNSCLC carcinomas and normal specimens, it was observed that thelevel of Egr-1 is less in the carcinomas than in adjacent normaltissue in more than 72% of the specimens (34). Our data showthat TGF- $beta$ ₁ stimulates expression of Egr-1 mRNA rapidly in NSCLCcells. It may be possible that Egr-1 may have growth inhibitoryproperties in NSCLC cells by stimulating secretion of TGF- $beta$ ₁,which in turn might act as an autocrine or paracrine agent toinhibit cell proliferation as in HT-1080 cells. However, becauseexpression of Egr-1 mRNA is only transient in NSCLC cells, thisinhibitory effect might be predicted to be transient as well.In contrast, TGF- $beta$ ₁ stimulates expression of Egr-1 mRNA in a morepersistent manner in NHBE cells so that the growth inhibitoryactivities of Egr-1 might be predicted to be more prolonged thanin NSCLC cells. Future studies will focus on whether this is thecase to better understand the mechanism of growth control by Egr-1in normal and malignant lung cells.

	Footnotes

Address correspondence to: Sonia B. Jakowlew, Ph.D., National Cancer Institute, Medicine Branch, Department of Cell and Cancer Biology, 9610 Medical Center Drive, Suite 300, Rockville, MD 20850.

(Received in original form November 19, 1996 and in revised form March 17, 1997).

Acknowledgments: The authors thank Dr. V. Sukhatme (University of Chicago) for the gracious gift of human Egr-1 cDNA. They also thank Dr. T.Curran (St. Jude Children's Research Hospital) for the kind giftof c-fos cDNA and Dr. S. W. Qian (National Cancer Institute) forTGF- $beta$ ₁ cDNA.

Abbreviations Egr-1, early growth response gene-1; NHBE, normal human bronchial epithelial; NSCLC, non-small cell lung cancer; PCR, polymerase chain reaction; PKC, protein kinase C; PMA, phorbol myristate acetate; TGF- $beta$ ₁, transforming growth factor- $beta$ 1.

	References

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