Zebrafish Agr2 Is Required for Terminal Differentiation of Intestinal Goblet Cells

Background Mammalian Anterior Gradient 2 (AGR2) is a protein disulfide isomerase that is required for the production of intestinal mucus and Paneth and goblet cell homeostasis. However, whether increased endoplasmic reticulum (ER) stress occurs in Agr2−/− mice remains a controversial issue. Methodology/Principal Findings We characterized the function of zebrafish agr2 by both morpholino antisense oligomer-mediated knockdown and agr2 mRNA overexpression. Fluorescent whole-mount double in situ hybridization indicated that in the intestine, agr2 was only expressed in goblet cells. Significantly increased numbers of immature Alcian blue-stained goblet cells were observed in the intestines of 104- and 120-hours post fertilization (hpf) agr2 morphants. Transmission electron microscopy analyses further confirmed the existence of immature pre-goblet cells containing few mucous granules in the mid-intestines of 104- and 120-hpf agr2 morphants. agr2 expression was not significantly induced by an ER stress inducer, tunicamycin. Expression of the ER chaperone gene hspa5, the spliced form of xbp1s, c/enhancer binding protein homologous protein chop, and the activating transcription factor 4b1 atf4b1 were not significantly induced in either 104-hpf agr2 morphants or agr2-overexpressed embryos. Similar percentages of P-Histone H3-stained M phase cells were identified in intestines of 104-hpf agr2 morphants and control embryos. Conclusions/Significance Our study demonstrates that in contrast to mouse AGR2, zebrafish Agr2 is expressed in only one intestinal secretory cell type - the goblet cells. Agr2 is essential for terminal differentiation of intestinal goblet cells in zebrafish embryos. Either knockdown of agr2 function or agr2 overexpression could not extensively induce expression of members of the unfolded protein response pathway.


Introduction
Anterior gradient 2 genes, such as XAG-1 and XAG-2, were first identified as cement gland-specific genes in Xenopus [1]. Studies have shown that the function of XAG-2 in ectodermal patterning is to specify the differentiation of the cement gland and forebrain [2]. Subsequently, anterior gradient 2 homologues have been identified in different vertebrates ranging from newts to mammals. Newt nAG was shown to play an essential role in the regeneration of the limb [3]. Two human homologues (HAGR2 and HAGR3) have been identified. They are located adjacent to one another on chromosome 7, and they share 71% amino acid sequence similarity [4]. Activated AGR2 expression was found in different human cancer cells including breast, prostate, ovarian, esophagus, gastro-intestinal tract and lung, indicating a role in promoting cell proliferation [5]. Knockdown of AGR2 expression in estrogen receptor-a-positive breast cancer cell lines inhibited cell growth and induced cell death by modulating expression of cyclin D1, estrogen receptor-a, and survivin [6]. Recent work demonstrated that human AGR2 promotes cell growth by modulating expression of amphiregulin, an EGFR ligand, and YAP1, a co-activator of the HIPPO pathway [7]. Furthermore, human AGR2 was considered to be a metastasis inducer because high incidences of metastases occurred in the lungs of animals receiving AGR2 transfectants [8].
Human AGR2 and AGR3 were later identified as novel members of the protein disulfide isomerase family [9]. They contain one thioredoxin (Tx)-domain motif (CXXC), which facilitates oxidation and reduction. HAGR2 and HAGR3 shared high amino acid similarity with ERp18/19 and contain reminiscence of an ER retrieval signal in their C-termini (KTEL and QSEL, respectively). The mouse homolog of Agr2, GOB-4, was shown to be strongly expressed in the adult small intestine, colon, and stomach [10]. Immunohistochemistry further demonstrated that mouse AGR2 was localized in proliferating intestinal stem cells/early progenitor cells (such as Musashi-1 (MSI1)-positive cells at the crypt base) and also in differentiated secretory cell lineages, including goblet, Paneth and enteroendocrine cells [11]. Both germline and inducible Agr2 2/2 mice were generated by two different studies to investigate AGR2 function in intestinal development [12,13]. Mouse AGR2 was demonstrated to localize to the lumen of the endoplasmic reticulum (ER) of intestinal secretory epithelial cells and is required for the production of mucin and mucus in the intestine [13]. Mouse AGR2 was also shown to be required to maintain homeostasis of both Paneth and goblet cells in the intestine [12]. Furthermore, mice lacking Agr2 were susceptible to colitis, suggesting a role in the protection from diseases such as inflammatory bowel disease. The results from mouse models and human inflammatory bowel disease demonstrated a close relationship between ER stress, activation of the unfolded protein response (UPR) and intestinal inflammation [14]. However, different results regarding whether ER stress is induced in the intestine of different Agr2 2/2 null mice were reported [12,13].
Zebrafish has been widely used as an important model organism for the study of gastrointestinal development and related human diseases [15]. Compared to the mammalian intestinal epithelium, zebrafish do not have either crypts of Lieberkuhn or Paneth cells. Zebrafish villi possess three different differentiated cell types, these include enterocytes, which are responsible for nutrient absorption; goblet cells, which secrete the mucus layer to protect the intestinal epithelium from pathogens; and enteroendocrine cells, which produce different hormones that maintain normal physiological function [16]. Previously, we cloned and characterized the zebrafish agr2 gene [17]. Whole-mount in situ hybridization demonstrated that agr2 is expressed in most organs that contain mucus-secreting cells, including epidermis, olfactory bulbs, otic vesicles, pharynx, esophagus, pneumatic duct, swim bladder, and intestine. In this study, both morpholino antisense oligomer knockdown and overexpression approaches were used to investigate agr2 function in intestinal development. Knockdown of agr2 expression caused defects in the maturation of intestinal goblet cells detected by both Alcian blue staining and transmission electron microscopy analysis. Either knockdown of agr2 function or agr2 overexpression could not extensively induce expression of members of the UPR pathway. Agr2 was not required for normal intestinal cell proliferation.

Zebrafish Maintenance and Staging
Wild type zebrafish AB strain was maintained as previously described [18]. Different developmental stages were determined as described [19]. All animal procedures were approved by the Animal Use and Care Committee of Academia Sinica (protocol # RFiZOOHS2009095).
To demonstrate the specificity of two agr2 translational MOs, we fused the agr2 MO sequence in front of the GFP start codon which is under the control of CMV enhancer/promoter. GFP expression patterns were examined for embryos that had been respectively injected with 100 pg of CMV-agr2 mo-GFP plasmid alone, coinjected with 3.9 ng each of agr2-MO1 and agr2-MO2 and 100 pg of CMV-agr2 mo-GFP plasmid or with 3.9 ng each of agr2-5 mmMO1 and agr2-5 mmMO2 and 100 pg of CMV-agr2 mo-GFP plasmid at 30 hpf.
Whole-Mount In Situ Hybridization, Fluorescent Whole-Mount Double In Situ Hybridization, Whole-Mount Immunohistochemistry, p-Histone H3 Immunostaining and Alcian Blue Staining Whole-mount in situ hybridization was conducted on embryos treated with 0.003% phenylthiocarbamide using digoxigeninlabeled antisense RNA probes and alkaline phosphatase-conjugated anti-digoxigenin antibodies as described previously [20].
For fluorescent whole-mount double in situ hybridization, fixed and dehydrated embryos were incubated with 2% H 2 O 2 in methanol for 20 min before rehydration and rinses in PBST (0.1% tween 20). After 40 min proteinase K (10 mg/ml) treatment, 20 min 4% paraformaldehyde fixation, and PBST washes, embryos were incubated in hybridization solution containing 5% (V/V) dextran sulfate and either fluorescein-or digoxigeninlabeled RNA probes at 65uC overnight. The next day, embryos were incubated in 5% serum for 1 h after RNA probe removal and washes. Embryos were then incubated with pre-absorbed horseradish peroxidase-conjugated anti-fluorescein antibody (1:500) diluted in 5% serum at 4uC for overnight. The next day, embryos were washed with PBST and rinsed with a solution containing 100 mM borate, pH 8.6 and 0.1% tween 20 and then incubated with reaction buffer (100 mM borate, pH 8.6, 2% (V/ V) dextran sulfate, 450 mg/ml 4-iodophenol, 0.1% tween 20, 0.003% H 2 O 2 ) containing TSA plus fluorescein reagent (1:100, Perkin Elmer) for 40 min. Embryos were then washed with PBST and the peroxidase reaction was inactivated by incubation in solution containing 100 mM glycine, pH 2.0 and 0.1% tween 20 for 10 min. Embryos were then blocked with 5% serum before incubation with horseradish peroxidase conjugated anti-digoxigenin antibody (1:500) at 4uC overnight. The next day, embryos were stained with reaction solution containing TSA plus Cyanine 3 reagent (1:100) for 40 min. Embryos were then washed with PBST, 50% methanol and 100% methanol, and incubated in 1% H 2 O 2 in methanol for 30 min before fixation in 4% paraformaldehyde. Embryos were then stored in 80% glycerol. Two templates were linearized, and antisense RNA probes were produced as follows: agr2 (Bam HI/T7) and glucagon (Nco I/SP6).
For whole-mount immunohistochemistry, embryos were fixed with 4% paraformaldehyde at 4uC for 3 h and then washed with PBS containing 0.1% triton x-100 and methanol. After rehydration, embryos were treated with proteinase K (10 mg/ml) for 40 min. Following PBST washes, embryos were incubated in 10% serum at room temperature for 1 h before incubation with antisalmon Agr2 antiserum diluted in blocking solution containing 5% serum and 2 mg/ml BSA (1:200) at 4uC overnight [21]. After PBST washes, embryos were incubated with Alexa 488-conjugated anti-rabbit secondary antibody (1:200) at room temperature for 3 h. Embryos were stored in 80% glycerol following PBST washes.
For tunicamycin treatment, 96-hpf wild type embryos were incubated in respective 1, 2 or 3 mg/ml of tunicamycin in DMSO for 24 h and harvested at 120 hpf for total RNA extraction. As a control, 96-hpf wild type embryos were treated with DMSO (5 mg/ml) for 24 h and total RNA were harvested at 120 hpf.
To synthesize 1 st -strand cDNA, a reaction buffer (15 ml) containing 1 mg total RNA and 500 ng random primer was heated at 70uC for 5 min and then chilled on ice. Reverse transcription reaction was then conducted by addition of 15 ml solution containing RT buffer (16 final concentration), MgCl 2 (2.5 mM final concentration), 1 ml RNase inhibitor, dNTP (0.5 mM final concentration), and 3 ml Impron II Reverse Transcriptase (Promega). Reverse transcription reaction was incubated at 25uC for 10 min, 55uC for 1 h and then heated at 70uC for 10 min. qPCR was conducted in a 20 ml reaction buffer containing 83.3 ng diluted cDNA, forward and reverse primer pair (each of 0.25 mM final concentration), and SYBR Green I (16 final concentration) using a Roche Light Cycler 480 II machine. PCR cycles are: 95uC 10 min; 95uC 10 sec, 60uC 10 sec, 72uC 10 sec for 45 cycles; 95uC 5 sec; 65uC 1 min; 4uC 30 sec. The agr2 primer pair was F: GGTCACGATCCAAGAACAAG and R: CCATCAGGAGACAAGTGCTT. The hspa5 primer pair was F: CGAAGAAGCCAGATATCGATGA and R: ACGGCTCTTT-TCCGTTGAAG. The xbp1s primer pair was F: TGTTGCGA-GACAAGACGA and R: CCTGCACCTGCT GCGGACT. The atf4b1 primer pair was F: CTTTCTCTCCTCCTGCTTCT and R: GAG TCACACGACCCAATCA. The chop primer pair was F: GAGTTGGAGGCGTGGTATGA and R: CCTTGGTGGC-GATTGGTGAA. The pdia5 primer pair was F: GGAGACG-TAGGAGACTGGT and R: CACATCAGACAGCAGCTT. The EF-1a primer pair was F: CTGGAGGCCAGCTCAAACAT and R: ATCAAGAGTAGTACCGCTAGCATTAC.

Histology, Photography, and Electron Microscopy
Cryostat sectioning of 104-hpf agr2 morphants, agr2-5 mmMO1 and 5 mmMO2-coinjected, and wild type embryos were performed as described [22]. Images of embryos were taken using either an RT color digital camera (SPOT) on a Zeiss Axioplan 2 microscope equipped with DIC mode or a Leica DFC 310 FX on a Leica Z16 Apo stereomicroscope. Fluorescent images were taken using a Leica TCS-SP5-MP confocal microscope. Transmission electron microscopy analysis was performed as described previously [18].

Zebrafish agr2 Is Exclusively Expressed in Intestinal Goblet Cells
Mouse AGR2 is expressed in MSI1-positive intestinal stem cells and in all three intestinal secretory cell lineages including goblet, Paneth and enteroendocrine cells [11]. There are no Paneth cells in the intestines of zebrafish. We performed fluorescent wholemount double in situ hybridization of zebrafish using agr2 and glucagon as probes. As shown in Figure 1, there is no overlapping expression between agr2-expressing goblet cells and glucagonexpressing enteroendocrine cells. This result indicates that in contrast to the expression of mouse AGR2 in all intestinal secretory cell lineages, zebrafish agr2 is solely expressed in intestinal goblet cells.

Morpholino Antisense Oligomer (MO)-Mediated Knockdown of agr2 Expression
To investigate agr2 function, two agr2-specific translational MOs (agr2-MO1 and agr2-MO2) were designed to inhibit its protein synthesis. Five mismatches were introduced in these two agr2-MOs and used as controls in this study. Initial experiments performed to determine the optimal required doses demonstrated that injection of 7.8 ng of agr2-MO1 (n = 61) or agr2-MO2 (n = 116) was required to achieve a high morphant rate (88.5% and 81.0%, respectively) as determined by Alcian blue staining (data not shown). However, coinjection of 3.9 ng each of agr2-MO1 and agr2-MO2 can obtain a similarly high (87.0%, n = 132) morphant rate. These results demonstrate that there is a synergistic effect between the two translational agr2-MOs. Therefore, we coinjected 3.9 ng each of agr2-MO1 and agr2-MO2 to generate agr2 morphants in the following experiments. Global morphology of agr2 morphants was similar to that of embryos that had been coinjected with agr2-5 mmMO1 and 5 mmMO2 and un-injected wild-type embryos at 24 or 104 hours post fertilization (hpf) (Figure 2A). To test the effectiveness of agr2-MOs in preventing the expression of agr2, we conducted whole-mount immunohistochemistry using antiserum against salmon Agr2 [21]. Agr2-expressing goblet cells were detected at 104 hpf in the mid-intestines of wild type embryos and in embryos that had been coinjected with both agr2-5 mmMO1 and 5 mmMO2 ( Figure 2B). No Agr2-expressing goblet cells were detected in intestines of 104 hpf agr2 morphants. To further demonstrate the specificity of the agr2-MOs, we fused the agr2-MO sequence in front of the GFP start codon. We detected no green fluorescence in 30-hpf embryos (n = 72) that had been coinjected with 3.9 ng each of agr2-MO1 and agr2-MO2 and 100 pg of CMV-agr2-mo-GFP expression plasmid ( Figure 2C). By contrast, bright GFP fluorescence was detected in 78% embryos (n = 59) that had been coinjected with the same amount of the agr2-5 mmMO1 and agr2-5 mmMO2 and CMV-agr2-mo-GFP expression plasmid as well as in 59% embryos (n = 58) that had been injected with CMV-agr2-mo-GFP expression plasmid alone. These results demonstrated the specificity of the two translational agr2-MOs used in this study.

Defects in the Maturation of Goblet Cells Were Detected in the Intestines of agr2 Morphants
To investigate the role of agr2 in the differentiation of goblet cells, we used Alcian blue staining to detect sulfated and carboxylated sialomucins in intestinal goblet cells. Differentiation of goblet cells involves the initial formation of pre-goblet cells containing few mucous granules that later become mature goblet cells which possess abundant mucous granules. We defined Alcian blue-stained goblet cells with an area equal to or larger than 29.2261.41 mm 2 (n = 10) as mature goblet cells and those with an area less than this value as immature goblet cells. Approximately 93% of the goblet cells were immature in intestines of 104-hpf agr2 morphants (n = 46), compared to 41% (n = 41) and 46% (n = 40) in intestines of agr2-5 mmMO1 and 5 mmMO2-coinjected and wild type embryos, respectively ( Figure 3A-D). A similarly high percentage (92%, n = 23) of immature goblet cells remained in intestines of 120-hpf agr2 morphants compared to 15% (n = 27) and 21% (n = 30) in intestines of agr2-5 mmMO1 and 5 mmMO2-coinjected and wild type embryos, respectively ( Figure 3E-H). However, total intestinal goblet cell number, including both mature and immature goblet cell numbers, was similar among 104-and 120-hpf agr2 morphants, agr2-5 mmMO1 and 5 mmMO2-coinjected embryos, and wild type embryos.
We used transmission electron microscopy to better define goblet cell ultrastructure in the mid-intestines of 104-and 120-hpf agr2 morphants, agr2-5 mmMO1 and 5 mmMO2-coinjected embryos and wild type embryos (Figure 4). In the mid-intestines of 104-and 120-hpf wild type and agr2-5 mmMO1 and 5 mmMO2-coinjected embryos, mature goblet cells with many mucous granules that group into swollen thecae can be detected, while in the mid-intestines of 104-and 120-hpf agr2 morphants, the majority of goblet cells were pre-goblet cells with a small number of mucous granules.
Taken together, these results demonstrate that agr2 expression is essential for terminal differentiation of goblet cells in the intestines of zebrafish embryos and overexpression of agr2 promotes mucin production.

Knockdown of agr2 Expression and agr2 Overexpression Do Not Induce Expression of Unfolded Protein Response (UPR) Pathway Members
Previous studies had different results regarding induction of ER stress in Agr2 2/2 mice, so we investigated whether perturbing agr2 expression will induce ER stress in zebrafish embryos [12,13]. To cope with ER stress, genes involved in the UPR pathway are induced. We investigated the mRNA expression levels of members of the UPR pathway, including the hspa5 gene, which encodes ER chaperone GRP78; c/enhancer binding protein homologous protein (chop); activating transcription factor 4b1 (atf4b1); and the spliced form of X box-binding protein 1 (xbp1s). Mildly increased expression levels (ranging from 1.1-1.3 fold) of hspa5, xbp1s and atf4b1 were identified in agr2 morphants when normalized to wild type or to agr2-5 mmMO1 and 5 mmMO2-coinjected embryos ( Figure 6A and Information S1). However, no alteration in chop expression level was detected, and the observed mild increases in gene expression levels of hspa5, xbp1s, and atfb1 did not reach statistical significance after a Student's t-test comparison. In addition, normal ER ultrastructure was observed in goblet cells of 104-and 120-hpf agr2 morphants (Insets in Figure 4). Similarly, no induction of expression of hspa5, xbp1s, atf4b1, and chop could be detected in 104-hpf agr2-overexpressed embryos when normalized to wild type or to lacZ-overexpressed embryos ( Figure 6B and Information S2). These results demonstrate that neither agr2 deficiency nor agr2 overexpression can induce ER stress and UPR in zebrafish embryos.
We also treated embryos with different concentration (1-3 mg/ ml) of tunicamycin, which inhibits ER protein glycosylation and induces ER stress. We measured respective expression level of xbp1s, hspa5, agr2, and protein disulfide isomerase family A, member 5 (pdia5), which is an ER quality control system component gene and EF1a control gene in 120-hpf embryos that had been respectively treated with different concentration of tunicamycin ( Figure 6C and Information S3). Mildly increased expression levels (ranging from 1.6-1.7 fold) of agr2 and pdia5 were identified in 3 mg/ml tunicamycin treated 120-hpf embryos, however the observed mild increases in gene expression levels did not reach statistical significance after one-way analysis of variance using Tukey's honestly significant different method. While significantly increased expression levels (ranging from 5.5-12.4 fold) of xbp1s and hspa5 were detected in 120-hpf embryos that had been treated with the same concentration of tunicamycin. These results indicate that agr2 expression was not significantly induced in response to ER stress.

Agr2 Is Not Required for Intestinal Cell Proliferation
Activated AGR2 expression was identified in different human cancer cells and human AGR2 was shown to promote cell growth [5,6,7], so we performed p-Histone H3 immunostaining to investigate the role of agr2 in zebrafish intestinal cell proliferation (Figure 7). A similar percentage of p-Histone H3-stained M phase cells were detected in the mid-and posterior intestines of 104-hpf agr2 morphants (2.98%, n = 5), agr2-5 mmMO1 and 5 mmMO2coinjected embryos (2.65%, n = 6) and wild type embryos (2.78%, n = 5). These results indicate that Agr2 is not required for intestinal cell proliferation in zebrafish embryos.

Discussion
In this study, we characterized the role of zebrafish Agr2 in intestinal cell proliferation and differentiation. Our loss-of-function and overexpression studies indicate that Agr2 is required for the terminal differentiation of goblet cells in zebrafish embryonic intestines.

Zebrafish Agr2 Is Required for Terminal Differentiation of Intestinal Goblet Cells
Although zebrafish Agr2 shared high (72-80%) amino acid sequence similarities with those of human and mouse AGR2 [17], its distribution in intestinal cell types is different than that of mouse AGR2. A previous study showed that mouse AGR2 is expressed in MSI1-positive intestinal stem cells and all intestinal secretory cell lineages including goblet, Paneth and enteroendocrine cells [11]. In contrast to mammalian intestines, zebrafish intestines only contain 2 secretory cell types, goblet and enteroendocrine cells, and 1 absorptive cell type, enterocytes [16]. Zebrafish intestines do not possess crypts of Lieberkuhn or Paneth cells. Fluorescent whole-mount double in situ hybridization further confirmed our previous finding that in zebrafish embryonic intestines, agr2 is exclusively expressed in goblet cells.
Using agr2-specific morpholino antisense oligomers to knockdown agr2 expression, we demonstrated that Agr2 is required for the maturation but not for the initial differentiation of intestinal goblet cells. Over 90% of goblet cells in both 104-and 120-hpf agr2 morphants are immature Alcian-blue stained goblet cells, while the total goblet cell number was the same in agr2 morphants and control embryos (Figure 3). Ultrastructural analyses on goblet cells in the mid-intestines by transmission electron microscope (TEM) further demonstrated the existence of immature pre-goblet cells containing few mucous granules in both 104-and 120-hpf agr2 morphants (Figure 4). In addition, a significant 1.3-fold increase in areas of mature Alcian-blue stained goblet cells was identified in intestines of 104-hpf agr2-overexpressed embryos, suggesting that agr2 overexpression promotes mucin production ( Figure 5). Overall, our results are consistent with a previous study showing that mouse AGR2 is essential for the production of mucin and intestinal mucus [13]. Owing to the lack of a suitable antibody which could recognize Muc2 in intestines of zebrafish embryos, we were not able to confirm changes in Muc2 protein level when agr2 expression was perturbed in zebrafish embryos. Mouse AGR2 localizes to the lumen of ER and is a member of the protein disulfide isomerase family, which is involved in mucin processing. Therefore, we investigated the role of zebrafish Agr2 in ER stress [13]. In contrast to previous studies in two different cell lines, agr2 expression was mildly (1.7 fold) induced upon 3 mg/ml tunicamycin treatment in zebrafish embryos ( Figure 6C) [12,23]. In addition, similar induction level (1.6 fold) of pdia5 gene which is involved in ER quality control/folding machinery was detected in 3 mg/ml tunicamycin treated zebrafish embryos ( Figure 6C). These results indicate that in contrast to xbp1s and hspa5, expression levels of PDI members such as agr2 and pdia5 were mildly induced, which did not reach statistical significant level in response to ER stress.
In agr2 knockdown embryos, we detected mildly (1.1 to 1.3-fold) increased expression levels in several members of the UPR pathway, including hspa5, xbp1s and atf4b1. These expression level increases did not reach statistical significance after a Student's ttest comparison ( Figure 6A). This result was in agreement with previous reports showing that mild increases in expression of Bip and XBP1s were observed in Agr2 siRNA knockdown SU86.86 and  HEK-293T cells [12,23]. Our results also support a previous study showing statistically insignificant increases in the expression levels of Hspa5, Ero1, Atf4, and Atf6 in Agr2 2/2 mice [13]. We also detected no alteration in expression levels of genes involved in ER degradation of misfolded proteins (ERAD) including ER degradation-enhancing a-mannosidase-like lectins 1 (EDEM1), calnexin and calreticulin in either agr2 knockdown or agr2 overexpressed embryos, these results are different from a previous report conducted in HEK-293T cells (data not shown) [23]. In contrast to the existence of ER stress-induced rough ER dilation in the intestinal goblet cells of Winnie or Eeyore mutant mice harboring a Muc2 missense mutation [24], our TEM results showed normal ER ultrastructure in agr2 morphants ( Figure 4). Overall, our results suggest that Agr2 may not play important roles in the control of ER homeostasis in zebrafish embryos.
Both ulcerative colitis and Crohn's disease, two forms of chronic human inflammatory bowel disease (IBD), were shown to contain reduced mucosal thickness and low numbers of goblet cells [25]. Muc2 knockout mice spontaneously developed a mild colitis and treatment with cytotoxic luminal agents like DSS led to severe colitis [26]. Similarly, Agr2-deficient mice were highly susceptible to DSS-induced colitis due to abnormalities in MUC2 synthesis Expression level of members of the UPR pathway (hspa5, xbp1s, atf4b1, chop) was not altered in agr2 morphants when normalized to wild type or to agr2-5 mmMO1 and 5 mmMO2-coinjected 104-hpf embryos by qPCR. (B) Expression of members of the UPR pathway (hspa5, xbp1s, atf4b1, chop) was not altered in agr2-overexpressed 104-hpf embryos when normalized to wild type or to lacZ-overexpressed embryos by qPCR. (C) agr2 expression level was not significantly induced upon 3 mg/ml tunicamycin treatment by qPCR. One-way analysis of variance and Tukey's honestly significant different method (T-method) were conducted among different genes after treatment with different concentrations of tunicamycin [27]. Different letters (a, b, c) indicate a statistically significant difference (p,0.05). Average gene expression in fold changes for respective gene is indicated. Error bars indicate the standard error. doi:10.1371/journal.pone.0034408.g006 [13]. In the future, it will be interesting to investigate if DSS treatment can promote development of intestinal inflammation in agr2 knockdown zebrafish embryos and the possibility of using agr2 deficient zebrafish as a model to study IBD.
Results of p-Histone H3 immunohistochemistry demonstrated that Agr2 plays no role in regulating intestinal cell proliferation in zebrafish embryos (Figure 7). Our finding is consistent with a previous study showing that no decreased proliferation in either the small intestine or the colon could be detected in germline Agr2 2/2 mice [12]. However, these results are inconsistent with studies in cancer cell lines showing that human AGR2 can promote cell growth by modulating expression of cyclin D1 and components of the EGF and HIPPO signaling pathways [6,7]. This discrepancy may be due to the abnormal status of cancer cells versus normal intestinal cells.
In conclusion, our loss-and gain-of-function studies demonstrate that zebrafish Agr2 functions like its mouse homolog in regulating terminal differentiation of intestinal goblet cells. However, Agr2 may not play important roles in the control of ER homeostasis in zebrafish embryos.

Supporting Information
Information S1 Raw qPCR data regarding expression levels of members of the UPR pathway in wild type embryos or embryos that had been injected with either agr2-5 mmMO1 and 5 mmMO2 or agr2 MO1 and MO2. Information S3 Raw qPCR data regarding expression levels of agr2, ef1a and members of the UPR pathway in untreated wild type or tunicamycin-treated embryos. Crossing point (Cp) values of respective ef1a, agr2, pdia5, xbp1s, hspa5, and b-actin detected in 120-hpf untreated wild type or embryos that had been treated with 1-3 mg/ml tunicamycin for 24 h are shown. NTC represents no template control. Result of one-way analysis of variance and Tukey's honestly significant deferent method (T-method) is also shown. (DOC)