Volume 16, Issue 5 (May 2018)                   IJRM 2018, 16(5): 305-314 | Back to browse issues page


XML Persian Abstract Print


Download citation:
BibTeX | RIS | EndNote | Medlars | ProCite | Reference Manager | RefWorks
Send citation to:

Kiani K, Movahedin M, Malekafzali H, Mirfasihi F, Sadati S N, Moini A, et al . Effect of the estrus cycle stage on the establishment of murine endometriosis lesions. IJRM 2018; 16 (5) :305-314
URL: http://ijrm.ir/article-1-1106-en.html
1- Valiasr Reproductive Health Research Center, Tehran University of Medical Sciences, Tehran, Iran
2- Department of Anatomical Sciences, Faculty of Medical Sciences, Tarbiat Modares University, Tehran, Iran. , movahed.m@modares.ac.ir
3- Department of Epidemiology and Biostatistics, School of Public Health, Tehran University of Medical Sciences, Tehran, Iran
4- Department of Pathology, Massoud Clinical Laboratory, Tehran, Iran
5- Department of Traditional Pharmacy, School of Traditional Medicine, Tehran University of Medical Sciences, Tehran, Iran
6- Department of Obstetrics and Gynecology, School of Medicine, Tehran University of Medical Sciences, Tehran, Iran
7- Department of Toxicology and Pharmacology, School of Pharmacy, Tehran University of Medical Sciences, Tehran, Iran
8- Department of Endocrinology and Female Infertility, Reproductive Biomedicine Research Center, Royan Institute for Reproductive Biomedicine, ACECR, Tehran, Iran
Full-Text [PDF 664 kb]   (790 Downloads)     |   Abstract (HTML)  (3424 Views)
Full-Text:   (1252 Views)
Introduction
 
Retrograde menstruation to the peritoneal cavity has been considered as the cause of endometriosis by Sampson’s theory (1). So far, researchers have established different animal endometriosis models in both primates and non-primates based on the mentioned theory (2-3). Primates like baboon exhibit spontaneous menstruation similar to human beings. However, they are expensive and their handling is rather a difficult task. Therefore, rodent endometriosis models are used in preclinical research due to their low costs, convenient handling and genetic similarity (2). Establishment of a reliable and standardized animal model of endometriosis is necessary for the evaluation of new drug effects and for explaining different aspects of pathology or etiology of this disease. For this purpose, we need a model which has more similarity to human endometriosis.
Induction of endometriosis in rodents can be achieved by transferring the uterine tissue samples surgically or by injection into the peritoneal cavity (4-7). In the majority of previous studies, either the endometrium layer or all layers of uterine tissue is implanted at proestrus phase and in some other studies, the estrus cycle is not mentioned (6).
Endometriosis is an estrogen-dependent disease and endometriotic lesions will have enough growth in presence of a high level of estrogen (10). In previous studies, most researchers used the endometrium or uterine tissues at proestrus or estrus phase (6, 11, 12). However, proestrus is a very short phase, and endometriotic lesions do not have enough time to be exposed to enough estrogen level. The estrogen level is rapidly decreased in late proestrus and estrus as compared with metestrus and diestrus phases (13). There is only one study that found the endometriotic lesions in proestrus and estrus is fast to heal compared to metestrus/diestrus rats. They showed the slow regression of endometriotic lesions when the endometrial tissue was implanted during the metestrus and diestrus cycle. Their findings suggest that it is better to use animals in the stage of metesrus/diestrus for endometriosis lesions (14).
One important issue in the establishment of the endometriosis model for preclinical studies is to follow up the endometriotic lesions during the drug administration. Some researchers used high-resolution ultrasound in order to follow up the lesions (15, 11), some researchers opened the abdominal wall of rats by surgery every 2 or 4 wk and they excluded the rats with regressed lesions (16-18) and some studies used laparoscopy for mice (14, 19). But unfortunately, we did not have access to high-resolution ultrasound or laparoscopy for mice in our country. In addition, opening the abdominal wall induces the inflammatory reactions and changes the peritoneal cavity environment and also it is dangerous for the mouse. Therefore, we need a reliable method for preparing endometriosis mouse model.
In this study, we tried to establish an autologous endometriosis mouse model based on endogenous estrogen level and analyze the influence of estrus cycle on the maintenance of endometriotic lesions in different time points.
 
Materials and methods
 
Animals
Fifty-two female NMRI (Naval Medical Research Institute) mice aged 10-16 wk with a body weight of 24-30 gr were used for experiments. The animals were housed in groups of five per cage under standard laboratory conditions within a temperature-controlled environment on a 12 hr light/dark cycle. They had free access to water and standard pellet food. The manuscript was prepared according to the ARRIVE Guidelines (20).
The housing of female mice without any exposure to male pheromones leads to the cessation of cycling. Urine-soaked beddings from males and also male vasectomized mice were transferred to the females' cages to synchronize and maintenance of estrus cycle in female mice, a phenomenon referred to as Whitten effect (21). The vaginal lavage method was used for the identification of the estrus cycle stage of individual animals. For this purpose, 50-100 µl of sterile ddH2O was carefully pipetted into the vagina and then transferred on a glass slide for examination under a light microscope (22) (Figure 1). The transplantation was either performed at proestrus/estrus or at metestrus/diestrus cycles.
 
Endometriosis model
The mice were randomly divided into two groups based on their cycle stage on the day of surgical induction of endometriotic lesions: group 1 (proestrus or estrus, n=28), group 2 (metestrus or diestrus, n=24). All mice were anesthetized using an intraperitoneal injection of 100 mg/kg Ketamine (Alfasan, Woerden-Holland) and 10 mg/kg Xylazine 2% (Alfasan, Woerden-Holland), diluted at 1:10 (v/v) in sterile distilled water (23). Subsequently, a 2-cm vertical midline incision was made 0.5-1.0 cm rostral to the vaginal opening, and both the uterine horns were exposed. The left uterine horn was ligated between the cervix and ovary and was removed and transferred into a sterile glass Petri dish containing 2-3 mL of sterile phosphate buffer solution (PBS). By inserting one blade of small scissors under a loop microscope (Olympus-SZ60, Tokyo, Japan), the horn was opened longitudinally and divided into 2 mm segments with a sterile biopsy punch in the glass Petri dish (5). These small uterine segments were sutured (without removing myometrium) onto the upper and lower parts of the inner surface of the abdominal wall (two to the right and two to the left side). Finally, the peritoneum and skin were closed with absorbable sutures. The mice were allowed to recover on a warm plate. All the operations were performed by a single researcher. The mice were analyzed after different implantation periods. Every 2 wk, some mice underwent an autopsy.
 
Macroscopic evaluation
For macroscopic evaluation, we assessed mean of lesions size and mean of macroscopic growth degree. Lesion size was calculated by multiplying the width and length of the lesions (expressed in mm2) measured by caliper and then mean of lesions size was measured per mouse. Macroscopic growth degree was calculated in accordance to Quereda and colleagues (24) with some modifications and classified in the following way: “degree 0-implantation disappears or absence of the cystic form; degree I-implantation forms a vesicle with a diameter smaller than 2 millimeters or solid form; degree II-implantation is cystic with fluid and its diameter is 2-4.5 mm; and degree III-vesicle with a diameter higher than 4.5 mm”. Cumulative macroscopic growth degree was calculated in each mouse. Degrees 0 or 1 were considered as an inadequate growth of lesions and degrees 2 or 3 were attributed to the adequate growth of lesions.
 
Histopathological examination and model success rate
The formalin-fixed endometriotic lesions were embedded in paraffin.sections (5-µm thickness) were stained with hematoxylin and eosin and examined under a light microscope. The endometriosis was diagnosed by identification of endometrial glandular tissue and stroma. The total model success rate was measured by dividing the total number of retrieved endometriotic lesions (confirmed by the pathology (by the total number of implanted uterine tissues multiplied by 100, which is expressed as a percentage. The individual peritoneal implant rate was defined as the number of retrieved endometriotic lesions (confirmed by pathology) divided by the number of implanted uterine tissues per animal multiplied by 100, which is expressed as a percentage.
 
Evaluation of persisting epithelium in endometrial autografts
Pathological evaluation of uterine autografts was performed by a semi-quantitative method, namely histopathological score (25) as following: “a well-preserved epithelial layer was scored 3, a moderately preserved epithelium with leukocyte infiltrate was scored 2, a poorly preserved epithelium (occasional epithelial cells only) was scored 1, and cases with no epithelium were scored 0”. Then mean histopathological score was calculated in each mouse.
 
Immunofluorescent analysis for apoptosis, cell proliferation, and vascularization of endometriotic lesions
Indirect immunofluorescence was used for immunohistochemistry. The endometriotic lesions were removed and fixed in formalin. They were then sectioned into 5 µm thick slices. The endometriotic lesion sections were fixed for 10 min in ice-cold acetone and were thereafter rehydrated in PBS containing 0.1% Triton X-100 for 5 min. The tissue was permeabilized and blocked in blocking solution containing 1% BSA/10% normal goat serum/0.3M glycine in 0.1% PBS-Tween for 1 hr. The sections were incubated overnight at 4oC with the following primary antibodies: rabbit polyclonal Caspase 3 (Abcam, ab4051) diluted 1:100 (for detection of apoptotic cells); rabbit polyclonal to Ki67 (Abcam, ab15580) diluted 1:100 (for detection of proliferating cells); rabbit polyclonal to Cd31 (Abcam, ab28364) diluted 1:100 (for detection of micro vessels in endometriotic lesions).
All dilutions were done in PBS containing 0.2% Triton X-100, 1% BSA and 2% normal goat serum. The sections were subsequently washed with PBS and incubated with goat-anti-rabbit Phycoerythrin (PE) conjugated (1:400; Invitrogen) as secondary antibody for 1 hr. at room temperature.  In addition, double staining was performed using DAPI (KPL) 1:5000. The same procedure was used for negative controls without using of primary antibodies.
Immunohistochemistry images were analyzed using the Image J software (http://rsbweb.nih.gov/ij/). The immune reactivity of the antibodies was visualized and photographed with an invert fluorescent microscope (Nikon, Japan) (200X). The fraction (percentage) of Ki67, CD31, and Caspase-3-positive cells was measured two sections per one lesion from each mouse at different estrus stages. All data were normalized to the area of endometriotic lesion section or the number of cells present in the lesion.
 
Ethical consideration
All the experiments were approved by the Ethics Committee of University of Medical Sciences, Tehran, Iran. The experiments were in agreement with Iran's Ministry of Health guidelines for the care and use of laboratory animals.
 
Statistical analysis
Data were expressed as mean ± standard deviation (S.D.). The data was first analyzed for normal distribution by SPSS software (Statistical Package for the Social Sciences, version 21.0, SPSS Inc, Chicago, Illinois, USA). Statistical analyses were performed using a Student’s t-test or Mann Whitney u-test for nonparametric data. p<0.05 were considered to be significant.



Figure 1. Cytological assessment of vaginal smears stained by Crystal Violet (A) Proestrus: epithelial cells-mostly rounded but some cells showing early stages of cornification of approaching estrus (B) Estrus: large cornified cells in clumps (C) Metestrus: leucocytes with smaller numbers of non-nucleated epithelial cells (D) Diestrus: mainly leucocytes with small number of nucleated epithelial and cornified cells. Scale bars: 10 µm.

Results
 
Macroscopic results
36 mice (69.2%) had visible lesions at the day of sacrifice. Two wk post-induction, there were small visible macroscopic lesions on the right or left peritoneum wall. Six wk post-implantation, all mice (100%) in metestrus/diestrus and 90.9% of mice at proestrus/estrus developed at least one cystic endometriotic lesion. The lesions appearance often was cystic with a homogenous surface. Our results showed that the factor `estrus cycle` did not significantly influence the size and macroscopic growth degree of endometriotic lesions at all observation time points (Table I). All endometriotic lesions were at degrees 2 or 3, which were considered as the adequate growth of lesions.
 
Histopathological examination and implant success rate
Typical histologic criteria of endometriotic lesions, including the presence of glandular epithelium and stromal elements, were confirmed in all lesions. Figure 2 shows the morphology and appearance of a peritoneal lesion after 6 wk of implantation. The endometriotic lesions of mice included a zone composed of 2 to 6 layer cells of endometrial stroma bearing scattered endometrial glands and an inner layer consisting of a single row of mostly columnar epithelial cells with occasional areas of pseudo-stratification. The lumen was filled with an amorphous eosinophilic material (Figure 3).
Histological characteristics of the remaining right uterine horn and the right ovary were normal without any evidence of endometriosis. Only acute inflammatory changes were observable in the perimetrium layer of uterine horn in some mice. From a total of 200 tissue samples sutured into the peritoneal cavity (109 tissue samples at proestrus/estrus and 91 tissues at metestrus/diestrus), 83 endometriotic lesions were confirmed by histopathology (overall model success rate of 41.5%). The model success rate for proestrus/estrus mice (phase1) was 60.7% vs. 79.2% for metestrus/diestrus (phase2) ones (p=0.229). The factor `estrus cycle` did not significantly influence the histopathological scores of endometriotic lesions (Table I).
 
Apoptosis, cell proliferation and vascularization in endometriotic lesions
Figure 4 shows a sample of immunocytochemistry sections from endometriotic lesions, indicating the expression of Caspase 3, ki67, and CD31 proteins. We could not found any significant difference in caspase-3-positive apoptotic cells of endometriotic lesions between two estrus cycles. In addition, the number of Ki67-positive stromal and glandular cells in endometriotic lesions and angiogenesis or vascularization of endometriotic lesions, which was indicated by CD31-positive micro vessels, was similar between two groups (Figure 5).


Table I. Results of autologous endometriosis models induced into the peritoneal cavity of 52 NMRI mice according to different estrus stages at operation day




Figure 2. The cystic endometriotic lesion on the right lower quadrant of peritoneum, 6 wk after implantation




Figure 3. H&E stained section of a cystic endometriotic peritoneal lesion, 6 wk after implantation, Magnification: 40×.



Figure 4. (A–F) Immunofluorescent sections of endometriotic lesions at proestrus/estrus (A, C, E) or at metestrus/diestrus stages (B, D, F), by fixation of uterine tissue samples to the peritoneal wall; Sections were stained with DAPI to identify cell nuclei (blue), an antibody against the apoptosis marker Caspase-3 (red) (A-B); and an antibody against the proliferation marker Ki67 (red) (C-D); an antibody against CD31 for the detection of the microvascular endothelium (red) (E-F). Magnification: ×200.



Figure 5. Caspase-3, Ki67 positive cells (%) and CD 31 positive micro vessels (%) in peritoneal endometriotic lesions at proestrus/ estrus (white bars) or metestrus/estrus (Grey bars) stages at operation day. Mean ± SEM.


Discussion
 
At present study, we used an autologous endometriosis mouse model without ovariectomy or any estradiol supplementation in order to mimic the human endometriosis and also we assessed the individual implant success rate of endometriosis as well as the change of endometriotic lesions during different stages of the estrous cycle in mice. Our results showed similar model success rate, similar macroscopic and histopathologic characteristics of endometriotic lesions at both estrus stages.
Endometriosis is an estrogen-dependent disease and endometriotic lesions will have enough growth in presence of a high level of estrogen (10). In previous studies, most researchers used the endometrium or uterine tissues at proestrus or estrus phase (6, 11-12). At late proestrus and estrus phase, the endometrial thickness of mice is higher than the other stages (26). This thickness may facilitate the endometrial sampling and provide enough tissue for suturing to the peritoneal wall. However, proestrus is a very short phase, and endometriotic lesions do not have enough time to be exposed to enough estrogen level. The proestrus phase of estrus cycle starts by increasing the 17-β-estradiol levels. This increment leads to indirect stimulation of gonadotropin-releasing hormone neurons in the hypothalamus and releasing luteinizing hormone and follicle-stimulating hormone into the circulation (22). In human, this phase is considered as follicular phase of the menstrual cycle (27). The peak in follicle-stimulating hormone levels stimulates the ovulation and estrus cycle will start. During estrus cycle, 17-β-estradiol decreases and prolactin has peak (22). In the other hand, metestrus/diestrus phases in mice are most comparable with the menstrual phase in humans and may be a suitable model for human endometriosis. Metestrus phase and increase amount of progesterone occur simultaneously and it is compatible with the start of human luteal phase (28). As progesterone levels begin to increase and there is a small spike in 17-β- estradiol levels in response to the activation of corpus luteum (28). Finally, entry into diestrus in mice happens and circulating progesterone levels peak. This phase is related to the human late luteal phase (29). Following a sharp decline in the level of progesterone, regression of the corpus luteum occurs (30).
Our results showed that the factor `estrus cycle` did not significantly influence the endometriosis size and macroscopic growth degree of endometriotic lesions in all four time transplantation periods. This finding is contrary to findings of Uchida and colleagues who found a correlation between the volume of endometriosis and the estrous cycle (14). Previous researchers have shown that endometriosis is a dynamic disorder causing spontaneous changes in lesion appearance, progression and regression over time (31). Endometriotic cysts regress with low estrogen levels, especially at estrus cycle, and reappear when the level of estrogen rises, especially at high estrogen levels (32). The estrogen level is rapidly decreased in late proestrus as compared with metestrus and diestrus phases (14). It means that maintenance of periodical sexual stages at mouse is more important than specific stage like proestrus or metestrus.
There was no significant difference in the mean histopathological scores between proestrus/estrus or metestrus/diestrus mice. Endometriotic lesions in all mice groups showed good or moderately preserved epithelial integrity with preserved well-ordered stroma. The presence of glandular epithelium is a hallmark and a diagnostic criterion for human endometriosis (25). This finding is similar to Wood and colleagues who showed that luminal epithelium proliferation, which was assessed by PCNA immunohistochemistry, was similar in different estrus stages (26). It means that this model can provide suitable and acceptable endometriotic lesions and can be comparable with the moderate stage of human endometriosis. In addition, all estrus stages showed adequate macroscopic growth of lesions according to Quereda and colleagues (24). 
In the present study, we also compared apoptosis, proliferation, and angiogenesis using immune histochemistry among two estrus cycle at operation day. We detected no difference with respect to cleaved Caspase-3-positive apoptotic cells, the number of neither Ki67-positive stromal and glandular cells nor angiogenesis or vascularization of endometriotic lesions, which was indicated by CD31-positive micro vessels in four time periods. It means that endometriosis model at both estrus stages prepare similar proliferation and similar angiogenesis for endometriotic lesions. Similar Ki67positive cells was also found in women with and without the endometriosis in three studies (33). In addition, similar apoptotic cells at endometriotic lesions in both groups suggest the reason for similar incidence and similar survival of endometriotic tissues at both estrus stages. Anti-apoptosis signaling and the acceleration of proliferation are typical molecular properties associated with the survival of endometriotic tissues (34-35). It is well established that endometriotic lesions need to gain a new blood supply to survive in ectopic sites, making angiogenesis essential for the development and establishment of endometriosis (36). Menstrual cycle phase has a significant effect on vessel segment length, both within each region and within uterus layers. However, we did not assess these findings in relation to estrous stage classification. Future studies should assess these factors in discrete estrus phases.
In most previous studies, either the endometriosis was implanted at proestrus phase or authors did not mention the estrus cycle (6). Furthermore, different methods such as homologous or heterologous were used. The lack of consistency with respect to estrogen supplementation, low and variable (30-50%) or unreported peritoneal implant success rates as well as model success rate are some other limitations of these studies (2, 37, 38). Establishment of a reliable and standardized animal model of endometriosis is necessary for the evaluation of new drug effects and for explaining different aspects of pathology or etiology of this disease. For this purpose, we need a model which has more similarity to human endometriosis. Our findings showed that we can use endometrium tissues at any estrus stages for autologous endometriosis mouse model.
 
Conclusion
 
In conclusion, these results show that the estrous cycle at operation day has no effect on the establishment and macroscopic or histological changes of ectopic endometriotic lesions at autologus endometriosis mouse model. If we maintain the endogenous estrogen levels in mice, we can induce endometriosis mouse model in both proestrus/estrus and metestrus/diestrus cycle without any significant difference.
 
Acknowledgments
 
This study was financially supported by Tehran University of Medical Sciences, Iran National Science Foundation and Royan Institute for Reproductive Biomedicine research center. The authors would like to thank the technicians of the Pathology Department at Massoud Clinical Laboratory. There is no conflict of interest in this study.
 
Conflict of interest
 
None Declared.
 
Type of Study: Original Article |

References
1. Sampson JA. Metastatic or embolic endometriosis, due to the menstrual dissemination of endometrial tissue into the venous circulation. Am J Pathol 1927; 3: 93-110.
2. Grummer R. Animal models in endometriosis research. Hum Reprod Update 2006; 12: 641-649. [DOI:10.1093/humupd/dml026]
3. Story L, Kennedy S. Animal studies in endometriosis: a review. ILAR J 2004; 45: 132-138. [DOI:10.1093/ilar.45.2.132]
4. do Amaral VF, Dal Lago EA, Kondo W, Souza LC, Francisco JC. Development of an experimental model of endometriosis in rats. Rev Col Bras Cir 2009; 36: 250-255. [DOI:10.1590/S0100-69912009000300012]
5. Pelch KE, Sharpe-Timms KL, Nagel SC. Mouse model of surgically-induced endometriosis by auto-transplantation of uterine tissue. J Vis Exp 2012; 59: e3396. [DOI:10.3791/3396]
6. Vernon MW, Wilson EA. Studies on the surgical induction of endometriosis in the rat. Fertil Steril 1985; 44: 684-694. [DOI:10.1016/S0015-0282(16)48988-0]
7. Körbel C, Menger MD, Laschke MW. Size and spatial orientation of uterine tissue transplants on the peritoneum crucially determine the growth and cyst formation of endometriosis-like lesions in mice. Hum Reprod 2010; 25: 2551-2558. [DOI:10.1093/humrep/deq201]
8. Hirata T, Osuga Y, Yoshino O, Hirota Y, Harada M, Takemura Y, et al. Development of an experimental model of endometriosis using mice that ubiquitously express green fluorescent protein. Hum Reprod 2005; 20: 2092-2096. [DOI:10.1093/humrep/dei012]
9. The Academy of Medical Sciences. Animals containing human material. London, The Academy of Medical Sciences; 2011.
10. Mihalyi A, Simsa P, Mutinda KC, Meuleman C, Mwenda JM, D'Hooghe TM. Emerging drugs in endometriosis. Exp Opin Emerg Drugs 2006; 11: 503-524. [DOI:10.1517/14728214.11.3.503]
11. Rudzitis-Auth J, Körbel C, Scheuer C, Menger MD, Laschke MW. Xanthohumol inhibits growth and vascularization of developing endometriotic lesions. Hum Reprod 2012; 27: 1735-1744. [DOI:10.1093/humrep/des095]
12. Laschke MW, Schwender C, Scheuer C, Vollmar B, Menger MD. Epigallocatechin-3-gallate inhibits estrogen-induced activation of endometrial cells in vitro and causes regression of endometriotic lesions in vivo. Hum Reprod 2008; 23: 2308-2318. [DOI:10.1093/humrep/den245]
13. Santmyire BR, Venkat V, Beinder E, Baylis C. Impact of the estrus cycle and reduction in estrogen levels with aromatase inhibition, on renal function and nitric oxide activity in female rats. Steroids 2010; 75: 1011-1015. [DOI:10.1016/j.steroids.2010.06.016]
14. Uchida M, Kobayashi O. Sequential observation of implanted endometriosis by laparoscopy in rats: correlation between the prevalence rate and the estrous cycle. J Pharmacol Sci 2013; 121: 299-304. [DOI:10.1254/jphs.12180FP]
15. Laschke MW, Körbel C, Rudzitis-Auth J, Gashaw I, Reinhardt M, Hauff P, et al. High-resolution ultrasound imaging: a novel technique for the noninvasive in vivo analysis of endometriotic lesion and cyst formation in small animal models. Am J Pathol 2010; 176: 585-593. [DOI:10.2353/ajpath.2010.090617]
16. Ergenoğlu AM, Yeniel AÖ, Erbaş O, Aktuğ H, Yildirim N, Ulukuş M, et al. Regression of endometrial implants by resveratrol in an experimentally induced endometriosis model in rats. Reprod Sci 2013; 20: 1230-1236. [DOI:10.1177/1933719113483014]
17. Güney M, Nasir S, Oral B, Karahan N, Mungan T. Effect of caffeic acid phenethyl ester on the regression of endometrial explants in an experimental rat model. Reprod Sci 2007; 14: 270-279. [DOI:10.1177/1933719107300911]
18. Nogueira Neto J, Coelho TM, Aguiar GC, Carvalho LR, de Araújo AG, Girão MJ, et al. Experimental endometriosis reduction in rats treated with Uncaria tomentosa (cat's claw) extract. Eur J Obstet Gynecol Reprod Biol 2011; 154: 205-208. [DOI:10.1016/j.ejogrb.2010.10.002]
19. Peterse DP, Fassbender A, O DF, Vanhie A, Saunders P, Vriens J, et al. Laparoscopic surgery: a new technique to induce endometriosis in a mouse model. Reprod Sci 2016; 23: 1332-1339. [DOI:10.1177/1933719116638178]
20. McGrath JC, Drummond GB, McLachlan EM, Kilkenny C, Wainwright CL. Guidelines for reporting experiments involving animals: the ARRIVE guidelines. Br J Pharmacol 2010; 160: 1573-1576. [DOI:10.1111/j.1476-5381.2010.00873.x]
21. Whitten WK. Modification of the oestrous cycle of the mouse by external stimuli associated with the male;changes in the oestrous cycle determined by vaginal smears. J Endocrinol 1958; 17: 307-313. [DOI:10.1677/joe.0.0170307]
22. McLean AC, Valenzuela N, Fai S, Bennett SA. Performing vaginal lavage, crystal violet staining, and vaginal cytological evaluation for mouse estrous cycle staging identification. J Vis Exp 2012; 67: e4389. [DOI:10.3791/4389]
23. Ricci AG, Olivares CN, Bilotas MA, Bastón JI, Singla JJ, Meresman GF, et al. Natural therapies assessment for the treatment of endometriosis. Hum Reprod 2013; 28: 178-188. [DOI:10.1093/humrep/des369]
24. Quereda F, Barroso J, Acien P. Individual and combined effects of triptoreline and gestrinone on experimental endometriosis in rats. Eur J Obstet Gynecol Reprod Biol 1996; 67: 35-40. [DOI:10.1016/0301-2115(96)02435-9]
25. Keenan JA, Williams-Boyce PK, Massey PJ, Chen TT, Caudle MR, Bukovsky A. Regression of endometrial explants in a rat model of endometriosis treated with the immune modulators loxoribine and levamisole. Fertil Steril 1999; 72: 135-141. [DOI:10.1016/S0015-0282(99)00157-0]
26. Wood GA, Fata JE, Watson KL, Khokha R. Circulating hormones and estrous stage predict cellular and stromal remodeling in murine uterus. Reproduction 2007; 133: 1035-1044. [DOI:10.1530/REP-06-0302]
27. Hawkins SM, Matzuk MM. The menstrual cycle: basic biology. Ann N Y Acad Sci 2008; 1135: 10-18. [DOI:10.1196/annals.1429.018]
28. Mihm M, Gangooly S, Muttukrishna S. The normal menstrual cycle in women. Anim Reprod Sci 2011; 124: 229-236. [DOI:10.1016/j.anireprosci.2010.08.030]
29. Sander VA, Facorro GB, Piehl L, Rubín de Celis E, Motta AB. Effect of DHEA and metformin on corpus luteum in mice. Reproduction 2009; 138: 571-579. [DOI:10.1530/REP-08-0325]
30. Rudolph M, Döcke WD, Müller A, Menning A, Röse L, Zollner TM, et al. Induction of overt menstruation in intact mice. PLoS One 2012; 7: e32922. [DOI:10.1371/journal.pone.0032922]
31. Harirchian P, Gashaw I, Lipskind ST, Braundmeier AG, Hastings JM, Olson MR, et al. Lesion kinetics in a non-human primate model of endometriosis. Hum Reprod 2012; 27: 2341-2351. [DOI:10.1093/humrep/des196]
32. Cason AM, Samuelsen CL, Berkley KJ. Estrous changes in vaginal nociception in a rat model of endometriosis. Horm Behav 2003; 44: 123-131. [DOI:10.1016/S0018-506X(03)00121-1]
33. Bourlev V, Volkov N, Pavlovitch S, Lets N, Larsson A, Olovsson M. The relationship between microvessel density, proliferative activity and expression of vascular endothelial growth factor-A and its receptors in eutopic endometrium and endometriotic lesions. Reproduction 2006; 132: 501-509. [DOI:10.1530/rep.1.01110]
34. Pellegrini C, Gori I, Achtari C, Hornung D, Chardonnens E, Wunder D, et al. The expression of estrogen receptors as well as GREB1, c-MYC, and cyclin D1, estrogen-regulated genes implicated in proliferation, is increased in peritoneal endometriosis. Fertil Steril 2012; 98: 1200-1208. [DOI:10.1016/j.fertnstert.2012.06.056]
35. Salmassi A, Acar-Perk B, Schmutzler AG, Koch K, Püngel F, Jonat W, et al. Apoptosis resistance in endometriosis. Bioimpacts 2011; 1: 129-134.
36. Rocha AL, Reis FM, Taylor RN. Angiogenesis and endometriosis. Obstet Gynecol Int 2013; 2013: 1-8. [DOI:10.1155/2013/859619]
37. Hsiao KY, Chang N, Lin SC, Li YH, Wu MH. Inhibition of dual specificity phosphatase-2 by hypoxia promotes interleukin-8-mediated angiogenesis in endometriosis. Hum Reprod 2014; 29: 2747-2755. [DOI:10.1093/humrep/deu255]
38. Nothnick WB, Graham A, Holbert J, Weiss MJ. miR-451 deficiency is associated with altered endometrial fibrinogen alpha chain expression and reduced endometriotic implant establishment in an experimental mouse model. PloS One 2014; 9: 1-11 [DOI:10.1371/journal.pone.0100336]

Send email to the article author


Rights and permissions
Creative Commons License This work is licensed under a Creative Commons Attribution-NonCommercial 4.0 International License.

Designed & Developed by : Yektaweb