Direct interaction between Rab5a and Rab4a enhanced epidermal growth factor-stimulated proliferation of gastric cancer cells

Guo-Jun Cao,Di Wang,Zhao-Pei Zeng,Guo-Xiang Wang,Chun-Jiu Hu,Zhi-Fang Xing

Guo-Jun Cao,Di Wang,Department of Laboratory Medicine,Huashan Hospital North,Shanghai Medical College,Fudan University,Shanghai 201907,China

Di Wang,School of Life Sciences,Fudan University,Shanghai 200433,China

Zhao-Pei Zeng,Department of Laboratory Medicine,Diniu(Shanghai)Health Technology Co.,Shanghai 201703,China

Guo-Xiang Wang,Department of Neurology,Institutes of Brain Science,State Key Laboratory of Medical Neurobiology and MOE Frontiers Center for Brain Science,Institute of Biological Science,Zhongshan Hospital,Fudan University,Shanghai 200032,China

Chun-Jiu Hu,Department of Gastroenterology,Ningbo First Hospital,Ningbo 315000,Zhejiang Province,China

Zhi-Fang Xing,Department of Laboratory Medicine,Huashan Hospital,Shanghai Medical College,Fudan University,Shanghai 200040,China

Abstract BACKGROUNDGastric cancer(GC)is one of the leading causes of cancer-related death worldwide.Although targeted therapies such as antibodies against human epidermal growth factor receptor 2 or vascular endothelial growth factor receptor 2 have been widely used in the treatment of metastatic cancer,the overall outcomes are poor.Therefore,elucidation of the mechanism underlying cancer progression is important to improve prognosis.Overexpression of the Rab5a gene has been confirmed to correlate with tumorigenesis of many cancers,but the mechanism underling,especially of GC,is still unclear.AIMTo investigate the effects of Rab5a overexpression on the tumorigenesis of GC.METHODSFirst,the expression levels of Rab5a and Rab4a in primary tumorous tissues of GC patients diagnosed between 2015 and 2018 were analyzed.Then we constructed HGC-27 cell lines overexpressing green fluorescent protein-Rab5a or red fluorescent protein-Rab4a and investigated the interaction between Rab5a or Rab4a using Western blotting,co-immunoprecipitation,confocal microscopy,and colocalization analysis.Finally,epidermal growth factor-stimulated proliferation of these cell lines was analyzed using cell counting kit-8 cell viability assay.RESULTSCompared with normal gastric tissues,the expression levels of Rab5a and Rab4a increased progressively both in paracancerous tissues and in advanced cancerous tissues.Epidermal growth factor could promote the proliferation of HGC-27 cells,especially Rab5a-overexpressing HGC-27 cells.Notably,Rab5a and Rab4a cooverexpression promoted the proliferation of HGC-27 cells to the greatest extent.Further analysis identified a direct interaction between Rab5a and Rab4a in HGC-27 cells.CONCLUSIONCo-overexpression of Rab5a and Rab4a in GC may promote the endosomal recycling of epidermal growth factor receptor,which in turn contributes to poor prognosis and tumor progression in GC patients.Inhibition of Rab5a or Rab4a expression might be a promising therapy for refractory GC.

Key Words:Rab4a;Rab5a;Epidermal growth factor;Cell proliferation;Gastric cancer;HGC-27 cell lines

INTRODUCTION

The incidence of gastric cancer(GC)in China ranks second only after lung cancer[1].It was reported that there are about 400000 new GC cases in China every year,accounting for 42% of the world’s total GC new cases[1].Although specific inhibitors against epidermal growth factor receptor(EGFR),vascular endothelial growth factor,and phosphatidylinositol 3-kinase signaling pathways have already been utilized in the treatment of GC,25%-40% of patients with stage II-IV GC still suffer from posttreatment recurrence[2-4].Therefore,there is an urgent need to elucidate the mechanism underlying GC progression for developing new drugs and improving prognosis.

Rab and Rab-related factors have been established as the main regulators of the activity of membrane trafficking and signal transduction pathways,which in turn regulate cell growth,survival,and programmed cell death or apoptosis[5-7].Among Rab and Rab-related factors,Rab5 was first found to be a member involved in sorting pathways and endocytic trafficking.There are three subtypes of Rab5 in eukaryotes,namely Rab5a,Rab5b,and Rab5c[7].These three subtypes can stimulate early endosome fusion and regulate the endocytosis of transferrin[8].Rab5a is highly expressed in human breast cancer[9],ovarian cancer[10],lung cancer[11],oral cancer[12],hepatocellular carcinoma[13],and gliomas tissues[14].Its overexpression is correlated with tumor malignancy and metastasis and may affect cell proliferation by regulating the activity of epidermal growth factor(EGF)signaling.Upon EGF stimulation,Rab5a can bind with its downstream effector PTB domain and leucine zipper motif 1(APPL1),which leads to the transportation of APPL1 from the cytoplasm to the nucleus,thereby improving cell proliferation[15,16].Rab4 includes three different subtypes:Rab4a,Rab4b,and Rab4c[17].Among these,Rab4a regulates the sorting and recycling of endosomes during membrane trafficking.Rab4a has also been implicated in the development of various types of cancer.For instance,Rab4a was found to be overexpressed in breast cancer and is believed to be involved in the rapid circulation of the invasive protein such as integrin and membrane-type 1 matrix metalloprotease[18].

Previous studies have found that Rab5a is significantly overexpressed in GC tissues,and that overexpression of Rab5a may be related to the advancement of GC[19-21].However,the underlying mechanisms remain unclear.To investigate the implication of Rab5a overexpression on GC development,in this study,we compared the expression levels of Rab5a and Rab4a in GC tissues with those in intestinal metaplasia tissue and surrounding normal gastric mucosa and found that the cancerous tissues exhibited significantly higher levels of Rab5a and Rab4a(P<0.01).Additionally,we found that Rab5a and Rab4a could directly interact with each other in HGC-27 cells.These results suggest that overexpression of Rab5a and Rab4a in GC may promote the endosomal recycling of EGFR,thereby enhancing the signal transduction and effects of EGF stimulation.This study may provide new ideas for the study of the occurrence and treatment of GC.

MATERIALS AND METHODS

Objectives

Primary tumor specimens were obtained from 42 GC patients who underwent resection between 2015 and 2018 in Huashan Hospital.Patients who had received chemotherapy or radiotherapy prior to surgery were excluded.The histological diagnosis was evaluated according to the World Health Organization guidelines[22].Clinical data were obtained from medical records.Patients aged from 32 to 81 years(60 ± 12 years,mean ± SD)were included in this study.The tumor stage was classified according to the eighth edition of tumor node metastasis(TNM)classification of the Union for International Cancer Control[23].Twenty patients(47.62%)were classified as early stage(stages I and II),while 22 patients(52.38%)were classified as advanced stage(stages III and IV)according to the clinical TNM.As for the histological grade,27 patients(64.28%)were graded as grade I or II,while 15(35.71%)were grade III or IV.With regard to metastasis,lymph node metastasis was observed in 22 patients(52.38%),while 20 patients(47.62%)were without metastasis.

Immunohistochemistry

All tissue sections were deparaffinized,rehydrated,and blocked as described by Crosbyet al[24].The sections were then incubated with antibodies(specified below)overnight at 4 °C.After washing with phosphate buffered saline(PBS),the sections were incubated with horseradish peroxidase-labeled goat anti-rabbit antibody(1:200;Santa Cruz Biotechnology,Dallas,TX,United States)for 1 h at room temperature.After repeated washing with PBS,the antigen-antibody complex was visualized with substrate chromogen(DAB;Dako Cytomation,Carpinteria,CA,United States)and counterstained with hematoxylin.Antibodies used in this study included rabbit polyclonal antibody against Rab5a,rabbit polyclonal antibody against Rab4a,rabbit polyclonal antibody against APPL1,and rabbit polyclonal antibody against histone deacetylase 1.All these antibodies were purchased from Santa Cruz Biotechnology.For grading purpose,the percentage of stained samples was determined based on immunohistochemical staining results.Samples in which no cell was stained were defined as “negative”.“Weak positive” was defined as <10% of the tumor cells positively stained,moderate positive was defined as 10%-50% of the tumor cells positively stained,and strong positive was defined as >50% of the tumor cells positively stained.

Construction and transfection of lentiviral plasmids

To construct a lentiviral plasmid overexpressing red fluorescent protein-Rab4a,upstream primer 5’-CCG GAATTC GCCACC ATGTCGCAGACGGCCATGTC-3’ and downstream primer 5’-CCG GGATCC CTAACAACCACACTCCTGAGCGTTC-3’ were used to isolateRab4acomplementary DNA(cDNA).Then the polymerase chain reaction products were digested and inserted into the pGMLV-mCherry-puro vector(Genomeditech Inc.,Shanghai,China).For the construction of lentiviral plasmid overexpressing Rab5a,two primers were synthesized,including 5’-CCG GAATTC GCCACCATGGCTAGTCGAGGCGCAA-3’ and 5’-CCG GGATCC TTAGTTACTACAACACTGATTCCTGGTTGGTT-3’,for amplification ofRab5acDNA.The polymerase chain reaction products were then digested and inserted into the pGMLVZsGreen1-Blasticidin vector(Genomeditech,Inc.).All the constructed plasmids were verified by Sanger sequencing at the Invitrogen DNA sequencing facility(Shanghai,China).HEK 293T cells were cultured in Dulbecco’s Modified Eagle Medium containing 10% fetal bovine serum,1 mg/mL puromycin,and 10 mg/mL blasticidin,penicillin and streptomycin.When cells reached 70%-80% confluence,they were cotransfected with aforementioned constructed plasmids using HG Transgene reagent(Genomeditech,Inc.)in accordance with the manufacturer’s protocol and maintained at 37°C for 48 h.For blank control,HEK 293T cells were transfected with the empty vectors(pGMLV-mCherry-puro or pGMLV-ZsGreen1-Blasticidin).The supernatant was harvested after 40 h.

Cell culture

Human GC cell line HGC-27 was purchased from the cell bank at the Institute of Biochemistry and Cell Biology(Shanghai Institute for Biological Sciences,Chinese Academy of Sciences,Shanghai,China).The cells were cultured in Roswell Park Memorial Institute 1640 medium supplemented with 10% fetal bovine serum(Gibco,Grand Island,NY,United States),streptomycin(100 μg/mL),and penicillin(100 U/mL)in a humidified atmosphere of 5% CO2at 37°C.For overexpression of green fluorescent protein-Rab5a or/and red fluorescent protein-Rab4a,HGC-27 cells were treated with the aforementioned supernatant containing lentiviruses.

Western blotting

Immunoblotting analysis was carried out using standard methods.Lysates prepared from control and transfected cells were separated by 10% sodium dodecyl sulfate polyacrylamide gel electrophoresis,and transferred onto polyvinylidene fluoride membranes(Millipore Corporation,Billerica MA,United States).The membranes were incubated with rabbit anti-human Rab5a(1:300)or Rab4a antibody(1:1000)overnight at 4℃.After washing polyvinylidene fluoride membranes with PBS,they were incubated with horseradish peroxidase-conjugated goat anti-rabbit immunoglobulin G(1:2000)for 2 h.After further washing,the immunoblots were developed using the enhanced chemiluminescence reagents(Amersham Life Science,Piscataway,NJ,United States).Each experiment was repeated three times.

Immunoprecipitation assay

Cell lysates were sonicated for 30 min before centrifugation at 12000 rpm for 10 min at 4°C.For co-immunoprecipitation,lysates were incubated with 20-40 μL of washed protein G agarose beads(Roche,Basel,Switzerland)for 3 h at 4°C to reduce nonspecific binding.Supernatants were incubated with primary antibodies for 2 h followed by the addition and overnight incubation with 20 μL of protein G agarose beads at 4°C with constant rotation.Last,samples were incubated at 95°C for 5 min with Laemmli buffer and subjected to immunoblotting.

Confocal microscopy and colocalization analyses

The transfected HGC-27 cell lines were cultured for live-cell confocal imaging on four- or eight-well chambered glass slides.Representative confocal images were recorded using Leica SP8 confocal microscope equipped with an HCX PL APO 63X/1.4 oil objective(Leica Microsystems,Wetzlar,Germany).Image acquisition was conducted at 1240 × 1240 pixels using sequential scanning for each channel.After background correction,RGB profile intensity and Manders’ correlation coefficient were used to measure the degree of colocalization between Rab5a and Rab4a with the EzColocalization tool in the National Institutes of Health ImageJ software(version:2.1.0/1.53c)[25].

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Cell proliferation assay

Viability of HGC-27 cells was measured using cell counting kit(CCK)-8(Dojindo,Rockville,MD,United States).Briefly,cells were seeded into six 96-well plates at the density of 1000 cells per well.For each cell line,two parallel samples were prepared,one was directly stimulated with 10 ng/mL EGF,the other remained untreated.The plates were cultured in a 5% CO2incubator at 37 °C.The proliferation of cells was evaluated at 0 h,24 h,30 h,48 h,54 h,and 72 h respectively by adding 5 μL CCK-8 solution(Fluka,Buchs,Switzerland)into each well.After that,the optical density of each well was measured at 450 nm and 630 nm using a microplate reader.All experiments were performed in triplicates.

Statistical analysis

All images were acquired using identical acquisition parameters,and all data are presented as means ± standard error.Significance was determined using student’sttest or Kruskal-Wallis Test.Values ofaP<0.05,bP<0.01,andcP<0.001 were considered indicative of significance.All statistical analyses were performed with R software packages,version 3.6.3(The R Foundation).

RESULTS

Rab5a and Rab4a were overexpressed in GC tissues compared with normal tissues

Our immunohistochemical staining analysis revealed “negative”(-)(Figure 1A and B)and “weak positive”(+)levels of Rab5a and Rab4a in normal and paracancerous gastric tissues,respectively(Figure 1C and D).In the epithelial cells of GC tissues,Rab5a and Rab4a were both overexpressed(+++)in the cytoplasm or on cell membrane(Figure 1E and F).

Figure 1 Microscopic images of immunohistochemical staining for Rab4a or Rab5a in gastric tissues.A and B:Negative(–)in normal tissue sections;C and D:Weak positive(+)in paracancerous tissue sections;E:Strong positive(+++);F;Moderate positive(++)in gastric cancer tissue sections.Original magnification:200 ×.

Figure 2 Expression levels of Rab5a and Rab4a in untransfected and transfected 293T cells.A:Expression level of Rab4a in 293T cells transfected with a plasmid overexpressing wild-type Rab4a.Untransfected 293T cells served as a Control group;B:Expression level of Rab5a in 293T cells transfected with a plasmid overexpressing wild-type Rab5a.Untransfected 293T cells served as a Control group.The asterisks indicate aP <0.05 compared with the controls.

The 42 GC specimens were classified into different clinical stages,and their immunohistochemical phenotypes were examined(Table 1):Among the 42 GC specimens,the overall Rab5a positive rate was 76.2%,while the overall Rab4a positive rate was 85.7%;among the 20 early-stage GC specimens,the Rab5a positive rate was 60.0%,and the Rab4a positive rate was 70.0%;the expression levels of Rab5a and Rab4a were further enhanced in advanced-stage GC specimens,with positive rates of 90.9% and 100% being observed for Rab5a and Rab4a,respectively.The difference between the two groups was statistically significant(P<0.05).Notably,the expression level of Rab5a increased from negative(-),to positive(+),to strong positive(++),and to very strong positive(+++)with the up stage of GC(P<0.01).For Rab4a,a similar trend was observed.Taken together,these data suggest that Rab5a and Rab4a may beinvolved in GC development.To verify these results,we further analyzed the expression patterns of Rab5a and Rab4a in normal gastric mucosa,gastric tissues adjacent to the tumors,early-stage GC tumor tissues,and advanced-stage GC tumor tissues.As shown in Table 2,the Rab5a and Rab4a positive rates were 20% and 10% in normal gastric mucosa,35.3% and 40% in adjacent tissues,60% and 70% in early-stage GC(I,II)tissues,and 90.9% and 100% in advanced-stage GC tissues,respectively.Moreover,the expression levels of Rab5a and Rab4a were significantly different among groups(P<0.01)(Table 2).Collectively,these results confirmed that the expression levels of Rab5a and Rab4a were progressively enhanced with the advancement of GC.In addition,similar trends were also observed for APPL1 and histone deacetylase 1 in normal gastric mucosa,gastric tissues adjacent to the tumors,earlystage GC tumor tissues,and advanced-stage GC tumor tissues with statistically significant differences(P<0.01)(Table 2).

Table 1 Expression levels of Rab5a and Rab4a in gastric cancer tissues with different clinicopathological characteristics

Table 2 Expression levels of Rab5a,Rab4a,leucine zipper motif 1,and histone deacetylase 1 in normal gastric mucosa,gastric tissues adjacent to the tumors,early-stage gastric cancer tumor tissues,and advanced-stage gastric cancer tissues as determined by immunochemical analysis

Overexpression of Rab5a and Rab4a in 293T cells

The lentiviral plasmids were first constructed to transfect transiently 293T cells;the expression levels of Rab5a and Rab4a were determined by western blot(Figure 2).After transfection,the level of Rab4a was significantly improved(Figure 2A),while that of Rab5a was moderately enhanced(about 5-8-fold as high as the endogenous expression level)(Figure 2B).The results showed that the endogenous Rab4a cannot even be detected by western blot in the 293T cell line(Figure 2A),while Rab5a expression is minimal(Figure 2B),and that the transfection was successful.

Overexpression of Rab5a and Rab4a enhanced EGF-stimulated HGC-27 cell proliferation

Before EGF administration,similar HGC-27 cell densities were observed in the Control group,Rab5a overexpression group,and Rab5a + Rab4a overexpression group.However,after 24 h of EGF stimulation,cell proliferation was found to increase significantly in all the groups.Among them,the Rab5a + Rab4a overexpression group had the highest cell density,followed by the Rab5a overexpression group,and finally the Control group(Figure 3A and B).There were statistically significant differences in cell density before and after(Figure 3A)EGF stimulation in all the groups(P<0.05).In addition,24 h after EGF stimulation,there were statistical differences between the Rab5a overexpression group and the Control group(P<0.05)and between the Rab5a + Rab4a overexpression group and the Rab5a overexpression group(Figure 3A)(P<0.05).

To characterize further EGF-stimulated HGC-27 cell proliferation,the cell viability of each group was then evaluated by CCK-8 assay as previously described[26].Upon EGF stimulation,cell proliferation in each group was increased significantly(Figure 3C,P<0.05).Among all the groups,the Rab5a + Rab4a overexpression group showed the largest increase in cell viability.These results indicated that Rab5a overexpression can significantly promote EGF-mediated cell proliferation,and this effect was further enhanced by Rab4a overexpression.

Figure 3 Overexpression of Rab5a and Rab4a promotes epidermal growth factor-induced proliferation of HGC-27 cells.Three groups of Control,Rab5a overexpression,and Rab5a + Rab4a overexpression were compared.Each group was analyzed with epidermal growth factor(EGF)or without(No-EGF)the presence of EGF treatment.A:A representative image of unstained cells(200 × magnification).The number in the upper right corner represents the cell concentration.Scale bar:50 μm;B:Analysis of HGC-27 cell concentration was performed using ImageJ software based on optical densities.Cell concentrations are expressed as percentages.The bars represent mean values and the mean ± standard error calculated based on 10 representative images from each group(n = 10).The asterisks indicate aP <0.05;C:Cell proliferation of each group was analyzed by cell counting kit-8 assay.The results showed that overexpression of Rab5a increased the proliferation of HGC-27 cells,and this effect was further enhanced by Rab4a overexpression.The asterisks indicate P <0.05(n = 3).

Rab5a directly interacted with Rab4a in HGC-27 cells

Under normal circumstances,HGC-27 cells express a low level of Rab5a and even a lower level of Rab4a(Figure 4A:a1-a4).We found that Rab5a overexpression resulted in a significantly increased level of endogenous Rab4a and that the two proteins colocalized in endosomes(Figure 4A:b1-b4).On the contrary,Rab4a overexpression did not significantly affect the protein level of Rab5a(Figure 4A:c1-c4).In HGC-27 cells of the Rab5a + Rab4a overexpression group,the two proteins co-localized in a large number of endosomes(Figure 4A:d1-d4).Quantitative analysis of the co-localization between Rab5a and Rab4a with ImageJ showed(Figure 4B)that despite background noises in the red and green fluorescence channels,a clear overlap between the two colors was observed.The above results suggest that Rab5a could directly interact with Rab4a to increase its protein level in HGC-27 cells.

In order to verify the aforementioned observations,we performed immunoprecipitation experiments in HGC-27 cells.As shown in Figure 5A and E,although Rab5a and Rab4a exhibited low endogenous expression levels in HGC-27 cells,an interaction between the two proteins was observed.This result confirmed a direct interaction between endogenous Rab5a and Rab4a proteins.In the Rab5a + Rab4a overexpression cells,a stronger interaction between the two guanosine triphosphatases was observed as expected(Figure 5D and H).Interestingly,in HGC-27 cells overexpressing Rab5a alone,although there is no artificial expression of Rab4a protein,the co-precipitation of Rab5a and Rab4a was still clearly observed(Figure 5B and F).On the contrary,in HGC-27 cells overexpressing Rab4a alone,the co-precipitation of Rab5a and Rab4a was weak(Figure 5C and G).Collectively,these results indicated that overexpression of Rab5a promoted the expression of endogenous Rab4a in HGC-27 cells and that the two proteins could directly interact with each other.

Figure 4 Confocal immunofluorescent analysis of the co-localization between Rab5a and Rab4a in endosomes of HGC-27 cells.A:Green fluorescent protein(GFP)–Rab5a and red fluorescent protein(RFP)–Rab4a overexpressed in HGC-27 cells were visualized using immunofluorescent confocal microscopy.Four groups of HGC-27 cells are shown,namely the Control group(a1-a4),the Rab5a overexpression group(b1-b4),the Rab4a overexpression group(c1-c4),and the Rab5a + Rab4a overexpression group(d1-d4).Scale bar = 20 μm;B:The colocalization between Rab5a and Rab4a was evaluated by EzColocalization plugin of ImageJ.Scatterplot of GFP–Rab5a and RFP–Rab4a is shown for cells in the Rab5a + Rab4a overexpression group(d4).

Figure 5 Rab5a could directly interact with Rab4a to regulate its protein level in HGC-27 cells.Lysates of untransfected HGC-27 cells(A and E)and HGC-27 cells transiently transfected with Rab5a(B and F),Rab4a(C and G),or Rab5a + Rab4a(D and H)were incubated with 20-40 μL of washed protein G agarose beads.Then the mixture was added with either anti-Rab4a antibody(upper row)or anti-Rab5a antibody(lower row).The immunocomplexes were resolved by sodium dodecyl sulfate polyacrylamide gel electrophoresis and were immunoblotted with either anti-Rab5a antibody(upper row)or anti-Rab4a antibody(lower row)as indicated.Results presented are representatives of at least three independent experiments.

Figure 6 Proposed schematic diagram of aberrant phenotype of endocytosis in cancer cells exhibiting enhanced cell proliferation and increased invasiveness.EGF;Epidermal growth factor;EGFR:Epidermal growth factor receptor;APPL1/2:Leucine zipper motif 1/2.

DISCUSSION

Rab proteins are small guanosine triphosphate-binding proteins.They belong to the largest Ras subfamily and are ubiquitously expressed in all eukaryotes[27].Rab5 protein was first cloned from a pheochromocytoma cDNA library by Zahraouiet al[28]in 1989.The first subtype was named Rab5a.Rab5a can stimulate early endosome fusion and regulate transferrin endocytosis[29,30].More studies have shown that overexpression of Rab5 is implicated human breast cancer[9],ovarian cancer[10],lung cancer[11],oral cancer[12],hepatocellular carcinoma[13],and gliomas[14].Rab4a is another subtype of Rab proteins.It is mainly located in the reticular coated vesicles,early endosomes,and circulatory endosomes and is an important regulator of endocytosis and circulation[31-34].It was found that the protein levels of Rab5a and Rab4a in malignant tumor cells were significantly higher than those in paracancerous tissues,which is consistent with the results of this study.Barbieriet al[29]found that EGF stimulation induced a specific,rapid,and transient activation of Rab5a in NR6 cells and that the activation of endocytosis by EGF was enhanced by expression of Rab5a,but not Rab5b or Rab5c.Similar to this finding,an inhibition on EGFR endocytosis had been observed by fluorescent assay in porcine aortic endothelial cells expressing a dominant negative Rab5a mutant and EGFR[35].Fukuiet al[36]found that Rab5a enhanced EGF-EGFR signal transmission in hepatocellular carcinoma and promoted the metastasis of hepatocellular carcinoma.Zhaoet al[10]found that EGF combined with EGFR could accelerate ovarian cancer cell proliferation through shuttling Rab5a and APPL1 from the plasmalemma into the nucleus.Yanget al[37]found that the increased expression of Rab5a protein in 123 breast cancer patients was associated with axillary LN metastasis.Tubbesinget al[38]found that Rab4 could increase EGFR activation in breast cancer cells.

In this study,we found that EGF can stimulate HGC-27 GC cell proliferation and that overexpression of Rab5a or Rab5a + Rab4a further enhanced the effect of EGF.Interestingly,the proliferation rate was the highest in the Rab5a + Rab4a group.The results of confocal microscopy suggested that Rab5a co-localized with Rab4a in endosomes.This observation was subsequently verified by our co-immunoprecipitation experiments,in which we found that Rab5a could directly interact with Rab4a in HGC-27 cells.There are very few reports about interaction between Rab5a and Rab4a[34,39].De Renziset al[40]discovered in 2002 that activated Rab5a could interact with Rab4aviarecruiting Rabenosyn-5 and a series of Rab effector proteins.

In conclusion,these results suggests that the interaction between EGFR and Rab5a is enhanced after EGF stimulation and that the direct interaction between Rab5a and Rab4a enhances the endosomal circulation of EGFR and thereby maintains its

expression level on the cell membrane.This can in turn enhance the effects of EGF,inc

CONCLUSION

Co-overexpression of Rab5a and Rab4a in GC may promote the endosomal recycling of EGFR,which in turn contributes to poor prognosis and tumor progression in GC patients.Inhibition of Rab5a or Rab4a expression might be a promising therapy for refractory GC.

ARTICLE HIGHLIGHTS

Research background

Gastric cancer(GC)is a common malignant tumor of digestive system with a poor overall prognosis.

Research motivation

The purpose of our study is to explore the pathogenesis of GC and improve the prognosis of GC.

Research objectives

We constructed HGC-27 cell lines overexpressing green fluorescent protein-Rab5a or red fluorescent protein-Rab4a and tissue samples of 42 patients with GC.

Research methods

Western blot,co-immunoprecipitation,immunohistochemistry,immunoprecipitation assay,cell culture,confocal microscopy,etc.were utilized.

Research results

Rab5a and Rab4a were overexpressed in GC tissues.The direct interaction between Rab5a and Rab4a enhanced epidermal growth factor-stimulated proliferation of GC cells.

Research conclusions

Co-overexpression of Rab5a and Rab4a in GC may promote the endosomal recycling of epidermal growth factor receptor,which in turn contributes to poor prognosis and tumor progression in GC patients.Inhibition of Rab5a or Rab4a expression might be a promising therapy for refractory GC.

Research perspectives

To explore the pathogenesis of GC and improve the prognosis of GC.

ACKNOWLEDGEMENTS

We thank Doctor Zhen Zhao(Minhang Hospital,Fudan University)for optimization of experimental scheme.