US20160066551A1

US20160066551A1 - Non human animal model for ulcerative colitis and its main complications

Info

Publication number: US20160066551A1
Application number: US14/943,422
Authority: US
Inventors: Eric Ogier-Denis; Xavier Treton; Fanny Daniel; Cecile Guichard; Eric Pedruzzi; Yoram Bouhnik; Yann Harnoy
Original assignee: Institut National de la Sante et de la Recherche Medicale INSERM
Current assignee: Institut National de la Sante et de la Recherche Medicale INSERM
Priority date: 2011-04-13
Filing date: 2015-11-17
Publication date: 2016-03-10
Also published as: WO2012140516A2; CA2832680A1; WO2012140208A1; WO2012140516A3; US20140031389A1; ES2607616T3; EP2696860B1; EP2696859A1; EP2696860A2; US9217156B2; JP2014512008A; CA2834960A1; US20140373186A1

Abstract

The present invention relates to a non human model animal for ulcerative colitis and its main complications such as primary sclerosing cholangitis and colorectal cancer. More particularly, the present invention relates to a transgenic non human animal model for ulcerative colitis and its main complications such as primary sclerosing cholangitis, and colorectal cancer comprising a targeted disruption in the IL10 and NOX1 genes so that IL10 and NOX1 are not expressed in said animal.

Description

FIELD OF THE INVENTION

The present invention relates to a non human model animal for ulcerative colitis and its main complications such as primary sclerosing cholangitis and colorectal cancer.

BACKGROUND OF THE INVENTION

Ulcerative colitis (UC) is a chronic intermittent and relapsing inflammatory bowel disease (IBD) of the colon characterized by superficial mucosal lesions that extend through the rectum and progress upstream. The natural history of UC is characterized by the progression of colonic lesions in up to 50% of subjects. This suggests that the colonic mucosa has a “global” susceptibility to environmental factors, but etiology of UC remains unknown and current treatments are limited as 30% of patients require colectomy. Human studies identified unbalanced endoplasmic reticulum stress (ERS) in unaffected colonic mucosa from UC patients^1,2. Animal models in which ERS is disrupted are highly sensitive to chemically-induced colitis ^2-6or develop intestinal inflammation ^2,7-9suggesting that unbalanced ERS give rise to inflammation. However, there are no ERS-regulating strategies proposed in the management of UC in part by the lack of adequate experimental model mimicking UC.

SUMMARY OF THE INVENTION

The present invention relates to a transgenic non human animal model for ulcerative colitis and its main complications such as primary sclerosing cholangitis, and colorectal cancer comprising a targeted disruption in the IL10 and NOX1 genes so that IL10 and NOX1 are not expressed in said animal.

DETAILED DESCRIPTION OF THE INVENTION:

The present inventors have generated a transgenic non human animal model of ulcerative colitis. They have found that a knock-out animal for IL10 and NOX1 results in a non-human animal which naturally develops a convincing ulcerative colitis phenotype, and its complications such as primary sclerosing cholangitis and colorectal cancer phenotype. Such animals allow compounds and other therapeutic regimens to be screened and evaluated in vivo as possible treatments or preventions for ulcerative colitis, primary sclerosing cholangitis, and colorectal cancer.
Accordingly, the present invention relates to a transgenic non human animal model for ulcerative colitis and its main complications such as primary sclerosing cholangitis, and colorectal cancer comprising a targeted disruption in the IL10 and NOX1 genes so that IL10 and NOX1 are not expressed in said animal.
As used herein the term “IL10 gene” has its general meaning in the art and refers to the gene encoding for interleukin 10 (IL10)
As used herein the term “NOX1 gene” has its general meaning in the art and refers to the gene encoding for NADPH-oxidase1 (Nox1).
The term “transgene” as used herein is intended to mean a nucleic acid vector which comprises nucleotide sequences which have been manipulated in-vitro and subsequently introduced into the genome of a species such that it is stably and heritably maintained in that genome. A “transgenic animal” is an animal that contains such a transgene within its cells.
Typically, the animal is a knock-out animal for IL10 gene and NOX1 gene. A “knock-out” animal is a sub family of transgenic animals, and is an animal wherein the transgenic construct has caused an endogenous gene not to be expressed.
The transgenic non-human animal of the invention may be any animal that initially comprises an endogenous NOX1 and IL10 gene. By endogenous is meant that the gene is comprised in the genome of that animal, and would under normal circumstances be expressed to produce the corresponding protein.
Preferably, the animal is a mammal. More preferably it is a rodent, and particularly preferred is when the transgenic animal is a mouse or a rat.
In a particular embodiment, the non human animal model is obtained by cross-breeding a knock-out animal for IL10 with a knock-out animal for NOX1.
The targeted disruption may be anywhere in the genes, subject only to the requirement that it inhibits expression of functional proteins. This may be achieved, for example, by inhibiting expression of the protein completely, or by causing expression of a truncated protein, or a protein that is mutated such that it cannot perform its function, for example by engineering amino acid mutations within the active site. Typically, the targeted disruption is such that a truncated, non-functional protein is translated by using an insertion of a stop codon into an exon. The targeted disruption of the gene locus is caused by the integration into the genome of the transgenic construct. Typically, the integration is achieved by homologous recombination.
Transgenic non-human animals of the invention may be produced by methods well known in the art. There are a number of techniques that permit the introduction of genetic material, such as a transgene, into the germline. The most commonly used, and preferred protocol comprises direct injection of the transgene into the male pronucleus of the fertilised egg, resulting in the random integration into one locus of a varying number of copies, usually in a head to tail array. The injected eggs are then re-transferred into the uteri of pseudo-pregnant recipient mothers. Some of the resulting offspring may have one or several copies of the transgene integrated into their genomes, usually in one integration site. These “founder” animals are then bred to establish transgenic lines and to back-cross into the genetic background of choice. It is preferable to have the transgene insertion on both chromosomes (homozygosity) as this obviates the need for repeated genotyping in the course of routine mouse husbandry.
Alternatively, for the production of transgenic mice, transgenes can be introduced via embryonic stem (ES) cells, using electroporation, retroviral vectors or lipofection for gene transfer. This is followed by the random insertion into the genome of the pluripotent embryonic stem (ES) cells, followed by the production of chimeric mice and subsequent germline transmission. Transgenes of up to several hundred kilobases of rodentian DNA have been used to produce transgenic mice in this manner.
The transgenic animals can be subsequently tested to ensure the required genotypic change has been effected, in any suitable fashion. This can be done by, for example, detecting the presence of the transgene by PCR with specific primers, or by Southern blotting of tail DNA with a specific probe. Testing for homologous recombination leading to insertion of the transgene is done by restriction digestion. The band sizes seen if recombination has taken place are different to those seen if it has not. Suitable methods for this procedure are given in the examples. Testing for homozygosity of the transgene insertion may be carried out using quantitative Southern blotting to detect a twofold difference in signal strength between hetero- and homozygous transgenic animals. Confirmation that the gene is not being expressed can be carried out by immunohistochemical techniques.
Once the desired genotype has been confirmed the transgenic animal line can be subjected to various tests to determine the phenotype as described in the Example. The tests involved in this phenotypic characterisation depend on what genotypic change has been effected, and may include, for example, morphological, biochemical and behavioural studies.
In one embodiment, the development of a colorectal cancer may be triggered by performing an appendectomy (or a caecal floor removing) on the transgenic non human animal. The inventors have indeed demonstrated that appendectomy (or a caecal floor removing) performed on a knock-out mouse for IL10 gene and NOX1 allows the reproducible development of a spontaneous colorectal cancer at age of 4-5 weeks.
The transgenic non-human animal model of the invention may be used to screen for drugs which reverse the phenotype demonstrated, and hence may be useful in treating or preventing ulcerative colitis and its main complications such as primary sclerosing cholangitis and colorectal cancer.
Accordingly a further object of the present invention relates a method for screening a candidate compound for use as a drug for the treatment or prevention of ulcerative colitis, and/or its mains complications such as primary sclerosing cholangitis or colorectal cancer comprising i) administering a transgenic non human animal model of the invention with the candidate compound, ii) characterizing the phenotype of the non human animal model of the invention after the administration of the candidate compound and iii) positively selecting the candidate compound that reverse or delay the phenotype of the non human animal model of the invention.
The method of the invention is thus particularly suitable for identifying dugs for the treatment of ulcerative colitis and/or for identifying drugs for the treatment and prevention f the main complications of ulcerative colitis such as primary sclerosing cholangitis or colorectal cancer.
The effect of the candidate compound on the transgenic non human animal model may be evaluated by determining whether the candidate compound causes a reversal, or ameliorates in any way any of the cellular or physiological changes caused by the disease (e.g. colitis, diarrhea, high incidence of rectal bleeding, change in body and colon weights, and prolapses). Typically, the candidate compounds can be tested using the assays and tests as described in the Example.
Suitable candidate compounds which may be tested in the above methods include antibody products (for example, monoclonal and polyclonal antibodies, single chain antibodies, chimeric antibodies and CDR grafted antibodies). Furthermore, combinatorial libraries, defined chemical identities, small molecules, peptides and peptide mimetics, oligonucleotides and natural product libraries, such as display libraries (e.g. phage display libraries) may also be tested.
In a particular embodiment, the candidate compound has been previously characterized as an inhibitor of PP1R15A/GADD34 which restores eIF2a phosphorylation.
Candidate compounds positively selected in the screening methods of the invention may be used to prevent or treat ulcerative colitis, primary sclerosing cholangitis and colorectal cancer. Accordingly, condition of a patient suffering from such a disease can therefore be improved by administration of such a product. The formulation of the product for use in preventing or treating the disease will depend upon factors such as the nature of the agent identified, the precise combination of symptoms, and the severity of the disease. Typically the agent is formulated for use with a pharmaceutically acceptable carrier or diluent. For example it may be formulated for intracranial, parenteral, intravenous, intramuscular, subcutaneous, transdermal or oral administration. A physician will be able to determine the required route of administration for each particular patient. The pharmaceutical carrier or diluent may be, for example, an isotonic solution. The dose of product may be determined according to various parameters, especially according to the substance used; the age, weight and condition of the patient to be treated; the route of administration; the severity of the disease, and the required regimen. A suitable dose may however be from 0.1 to 100 mg/kg body weight such as 1 to 40 mg/kg body weight. Again, a physician will be able to determine the required route of administration and dosage for any particular patient.
The present invention also provides a kit for screening a candidate compound for use as a drug for the treatment or prevention of ulcerative colitis, primary sclerosing cholangitis and colorectal cancer, which kit comprises a non-human animal model of the invention, and means for determining whether the candidate compound can ameliorate the phenotype of the non human animal model.
The invention will be further illustrated by the following figures and examples. However, these examples and figures should not be interpreted in any way as limiting the scope of the present invention.

EXAMPLE

Ulcerative colitis (UC) is characterized by exclusive colonic involvement with superficial mucosal lesions associated with depletion in goblet cells and decreased secretion of mucins in inflammatory colonic mucosa¹¹. Although it has been proposed that the epithelium of UC patients is diffusely abnormal irrespective to inflammation¹², early alterations predating inflammation within colonic epithelial cell remain elusive. It is now evident that impairment of proper ERS resolution by altered unfolded protein response (UPR) in epithelial cells can lead or sensitize to colonic inflammation both in animal^2-8and human studies^1,2. However, the consequences of ERS alterations during UC remain misunderstood. The UPR is a carefully orchestrated process involving three proximal sensors PERK, ATF6, and IRE1 that allow cells to cope with a wide variety of stressful conditions. The combined action of these sensors restores cell homeostasis by cessation of protein translation, increase of chaperones production, and degradation of the burden of aberrant proteins. Sustained or abnormal ERS adversely affects normal cell function leading to inflammation and/or apoptosis^13,14.
The relationship between goblet cells, ERS, and inflammation is unclear although goblet cells and mucus barrier have been linked to inflammation. However, knockout of the mucin gene Muc2 in mice is not sufficient to cause colitis since inflammation appears to arise only on a permissive genetic background^15,16and patients with UC express MUC2. Furthermore, partial or total depletion in the number of goblet cells^17-20and therefore in mucus and antibacterial products is insufficient to induce colitis. Finally, accumulation of missense mutated Muc2^ref.7or HLA-27 protein⁹which is prone to misfolding in the ER, or knockout of the protein disulfide isomerase Agr2^ref.5induce exaggerated ERS in secretory cells and subsequent inflammation. Thus, the predisposition to colitis might reside in goblet cells themselves and in their inability to manage ERS in the absence of immune dysfunction and in the setting of a normal colonic flora.
To explore the puzzling way by which goblet cells are affected by ERS in UC, we artificially increased the number of goblet cells in conditions of ERS. We crossed Nox1-deficient mice, which exhibit fine deregulation of colonic progenitor cells leading to increased goblet cell expression¹⁰, and IL-10^KOmice, which express deregulated ERS in epithelial intestinal cells⁸and develop enterocolitis depending on both genetic background and environmental factors²¹. The relevance of this IL-10/Nox1^dKOmodel relies on the human colonic epithelial cell expression of both IL-10²²and NOX1^23,24. Interestingly, NOX1 expression follows the same colonic gradient than goblet cells²⁵and UC lesions. Moreover, genome-wide association study demonstrate significant association of the small GTPase Rac1^ref.26(a partner of NOX1^ref.27) and IL-10 genes²⁸with UC. Here we showed that IL-10 and NOX1 expression levels were markedly altered in uninflamed colonic mucosa from patients with UC (n=12) versus healthy controls (n=12).
All SPF-reared C57B1/6-IL10/Nox1^dKOmice developed spontaneously colitis at 6/7 weeks and disease activity index (DAI) scores which became more severe with age, including diarrhea, high incidence of rectal bleeding, change in body and colon weights, and prolapses. None of WT and single-KO mice developed colitis during the time frame studied. Histopathologic scores revealed that IL10/Nox1^dKOmice developed more severe colitis along the proximal-distal axis and exhibited signs of UC without any signs of ileitis including polymorphonuclear infiltrates, crypt abscesses, edema, focal epithelial erosion, and crypt loss. We next measured epithelial permeability of FITC-dextran in segments of distal colon and indigenous bacterial translocation was identified in the spleen of 7 and 12-week-old mice. Consistent with the colitis state, only IL10/Nox1^dKOmice demonstrated an increased permeability in the colon and exhibited splenomegaly which was closely correlated with increased Gram-negative commensal bacteria translocation. Interestingly, IL10/Nox1^dKOmice showed the main complications of UC such as colitis-associated colorectal cancer and spontaneously primary sclerosing cholangitis at 7/8 months of age. By contrast, IL10^KOmice showed mild enterocolitis at low frequency (<20% at 34 weeks), without showing any signs of cholangitis or colorectal cancer (at >8 months of age; this study and²⁹). Interestingly, here we report the comprehensive genome-wide screen of 561 microRNAs of colonic epithelial mucosa of Nox1^KO, IL10^KO, and IL10/Nox1^dKOmice (6- and 16-wk-old) versus WT mice. Consistent with previous findings in patients with UC^30,31, IL10/Nox1^dKOmice expressed almost 50% of microRNAs relevant in defining UC signature.
To analyze cytokine responses at the site of inflammation, colon samples were collected and various cytokines were analyzed at both mRNA and protein levels. IL10/Nox1^dKOmice showed increased expression levels of pro-inflammatory cytokines mainly involved in UC. Lymphoid and myeloid cell population analysis in the spleen did not differ between the four genotypes. By contrast, a massive infiltration of FoxP3⁺T_regwas only observed in the colonic tissue in spite of active mucosal inflammation and at lesser extent in the spleen of IL10/Nox1^dKOmice consistent with findings in UC³². To determine whether the genotype of hematopoietic lineages affected the extent of colitis, we generated bone marrow (BM) chimeric mice in which recipients and donors were WT (CD45.1) and WT, IL10^KO, and IL10/Nox1^dKOmice (CD45.2), respectively. Interestingly, reconstitution of irradiated WT mice with IL10^KOor IL10/Nox1^dKOBM was insufficient to cause disease demonstrating that colitis is chiefly inherent to epithelial cells rather than hematopoietic lineages in IL10/Nox1^dKOmice.
The colonic epithelium of IL10/Nox1^dKOmice showed a paucity of Alcian Blue/PAS positive mucins associated with loss of goblet cells at the ulcerated sites. Accordingly, Muc2 and Muc4 protein expression levels were dramatically low in the inflamed colonic areas of IL10/Nox1^dKOmice. Rarefaction and aberrant morphology of goblet cells with few and immature thecae associated with small amount of mucus and swollen, round mitochondria were similarly observed in the colon of both IL10/Nox1^dKOmice and patients with UC.
Colonic section of IL10/Nox1^dKOmice displayed an increase in the number of PCNA- and phospho-histone 3-positive cells suggesting increased epithelial proliferation. Scanning electron microscopy (SEM) showed a ˜30% increase in crypt length in IL10/Nox1^dKOmice. Interestingly, SEM displayed a wide spectrum of identical ultrastructural alterations of the mucosa both in IL10/Nox1^dKOmice and in unaffected colonic mucosa of patients with UC including crypt distortion, visible crypt openings disposed in rows, edematous glandular borders, and dilatation of the gland lumen. Notwithstanding increased colonic proliferation, staining and quantitative assessment of apoptotic cells indicated that decreased expression of goblet cells in IL10/Nox1^dKO) mice was due to increased apoptosis in the colon.
To assess the pathogenic role of goblet cells in UC, WT and Nox1^KOmice were subjected to oral administration of DSS or rectal administration of TNBS. No significant differences in DAI and histological damages of colonic mucosa were seen between the two mouse models suggesting that chemically-induced inflammation is likely independent of increased expression of goblet cells. By contrast, tunicamycin treatment, a canonical inducer of ERS, significantly induced a more severe colitis in mice overexpressing goblet cells than in WT mice indicating that goblet cell itself may be a direct participant in the development of colitis as a consequence of ERS. Accordingly, IL10/Nox1^dKOmice exhibited ERS disturbances in the colonic mucosa prior inflammatory damages as previously described in patients with UC¹. IRE1beta and ATF6alpha branch signaling were extended in colonic epithelial cells as evidenced by the increased XBP-1 mRNA splicing, the induction of GRP78, GRP94, PDI at both mRNA and protein levels, and dilated cisternae and gross distortion of the ER in goblet cells. Interestingly, identical defective phosphorylation of eIF2α correlated with low expression of ATF4 was observed both in unaffected colonic mucosa of IL10/Nox1^dKOmice and patients with UC¹. Consistent with reduced eIF2α phosphorylation, increased expression of PPP1R15A/GADD34, a stress-inducible protein that recruits the catalytic subunit of protein phosphatase 1 and promotes eIF2alpha dephosphorylation, was detected in agreement with our previous data in humans¹. EIF2alpha phosphorylation is cytoprotective during ERS, because cells are sensitized to cell death when this pathway is genetically ablated³³and protected when it is ectopically enforced³⁴. To test whether a selective pharmacological inhibitor of GADD34-mediated eIF2alpha dephosphorylation may alleviate colitis, IL10/Nox1^dKOmice were treated with 1 mg/kg salubrinal³⁵for up to three weeks. We showed that salubrinal strongly reduced histological colitis score throughout the colon, markedly prevented immune cell infiltration, and restored intact mucosal architecture with normal goblet cells. Salubrinal caused robust eIF2alpha phosphorylation and protected colonic mucosa against apoptosis at least in part for its anti-apoptotic activity on CHOP expression. Furthermore, there was a trend toward reduced Grp78/Bip and Grp94 expression in salubrinal-treated mice demonstrating that salubrinal engages the translational control arm of the UPR by inducing eIF2alpha phosphorylation and acts like a proteostasis regulator by lowering protein folding in stressed cells. Interestingly, we demonstrated that salubrinal-induced phosphorylation of eIF2alpha was mainly detected in colonic epithelial cells. Finally, levels of proinflammatory cytokines and amount of colonic and splenic T_regcells were strongly decreased to baseline in salubrinal-treated IL10/Nox1^dKOmice.
Our findings strengthen that defective eIF2alpha phosphorylation is a major player in UC and may open new therapeutic avenues. Current treatments of UC cannot change the natural course of the disease. These difficulties to manage UC may be explained by the use of immunomodulators which are mainly designed to modulate the activity of immune cells and are hardly efficient to repair early epithelial abnormalities. Thus, eIF2α modulators could define a new class of drugs specifically based on the intimate mechanisms of UC which might likely shift the paradigm for UC treatment from immunomulators to epitheliomodulators.

REFERENCES

Throughout this application, various references describe the state of the art to which this invention pertains. The disclosures of these references are hereby incorporated by reference into the present disclosure.
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Claims

1. A transgenic non human animal model for ulcerative colitis and its main complications comprising a targeted disruption in the Interleukin 10 (IL10) and NADPH-oxidasel (NOX1) genes so that IL10 and NOX1 are not expressed in said animal.

2. The transgenic non human animal model according to claim 1 which is knock-out for IL-10 and NOX1.

3. The transgenic non human model according to claim 1 which is a rodent.

4. The transgenic non human model according to claim 1, wherein an appendectomy or a caecal floor removing was performed on the animal.

5. A method for producing a transgenic non human animal model for ulcerative colitis and its main complications, comprising cross-breeding a knock-out animal for IL10 with a knock-out animal for NOX1.

6-7. (canceled)

8. The transgenic non human animal model of claim 1, wherein said main complications include primary sclerosing cholangitis and colorectal cancer.

9. The transgenic non human animal model of claim 3, wherein said rodent is a mouse or a rat.