Microbiome analysis in women with endometriosis: Does a microbiome exist in peritoneal fluid and ovarian cystic fluid?

Abstract Purpose To investigate the relationship between the microbiome of the female genital tract and endometriosis. Methods This prospective cohort study included 36 women who underwent laparoscopic surgery for ovarian tumor from July 2019 to April 2020. Of them, 18 had endometriosis, and 18 did not have endometriosis. Vaginal secretions, endometrial fluid, peritoneal fluid, and ovarian cystic fluid were collected during surgery. Next‐generation sequencing of bacterial 16S rRNA was performed to characterize the microbiome. Results Specific microbiomes were not detected in either peritoneal fluid or ovarian cystic fluid regardless of the presence or absence of endometriosis and the type of cyst. When the cutoff value of infectious bacterial abundance in the vagina was set as 64.3%, there were many cases more than a cutoff value in the endometriosis group significantly (p = 0.01). When the cutoff value of infectious bacterial abundance in the endometrium was set as 18.6%, there were many cases more than a cutoff level in the endometriosis cases significantly (p = 0.02). Conclusion Peritoneal fluid and ovarian cystic fluid are almost sterile, although dysbiosis may occur in the vaginal and endometrial microbiome in women with endometriosis

Peripheral Opioid Antagonist Enhances the Effect of Anti-Tumor Drug by Blocking a Cell Growth-Suppressive Pathway <i>In Vivo</i>

<div><p>The dormancy of tumor cells is a major problem in chemotherapy, since it limits the therapeutic efficacy of anti-tumor drugs that only target dividing cells. One potential way to overcome chemo-resistance is to “wake up” these dormant cells. Here we show that the opioid antagonist methylnaltrexone (MNTX) enhances the effect of docetaxel (Doc) by blocking a cell growth-suppressive pathway. We found that PENK, which encodes opioid growth factor (OGF) and suppresses cell growth, is predominantly expressed in diffuse-type gastric cancers (GCs). The blockade of OGF signaling by MNTX releases cells from their arrest and boosts the effect of Doc. In comparison with the use of Doc alone, the combined use of Doc and MNTX significantly prolongs survival, alleviates abdominal pain, and diminishes Doc-resistant spheroids on the peritoneal membrane in model mice. These results suggest that blockade of the pathways that suppress cell growth may enhance the effects of anti-tumor drugs.</p></div

Blockade of OGF signaling by methylnaltrexone (MNTX) increased the growth of a diffuse-type GC cell line, but not an intestinal-type GC cell line, under low nutrient conditions.

<p>A, RT-PCR analyses of <i>PENK</i> and <i>OGFR</i> in diffuse-type GC cell lines, HSC-60 cells and highly metastatic 60As6 cells, 60As6 xenograft (60As6 xeno) and the intestinal-type GC cell line HSC-42. B, growth of 60As6 cells treated with OGF (10^-4 M), methylnaltrexone (MNTX, 10^-6 M), or a combination of these compounds for 72 h (mean ± SD, n = 3–6 per group, *<i>p</i><0.05, control vs. OGF, #<i>p</i> <0.05, OGF vs. OGF/MNTX). C, western blot analysis of OGFR protein in 60As6 cells with a stable transfectant of <i>OGFR</i> shRNA or control shRNA. D, growth of the stable transfectant of <i>OGFR</i> shRNA of 60As6 cells in the presence or absence of OGF (10^-4 M) for 72 h. Non-targeting control shRNA was used as a control (mean ± SD, n = 3 each). Growth of 60As6 cells (E) and HSC-42 cells (F) treated with MNTX (10^-6 and 10^-5 M) or a vehicle for 72 h under normal nutrient (10% FBS) and low nutrient (2% FBS) conditions. (mean ± SD, n = 4 each, *<i>p</i><0.05, vs. control).</p

Combined use of Doc and MNTX significantly prolonged survival and alleviated abdominal pain in model mice.

<p>A, survival curves of middle-phase peritoneal metastasis model mice treated with saline, Doc, or Doc/MNTX (0.3 mg/kg) (n = 5, *<i>p</i><0.05, vs. saline, #<i>p</i><0.05, Doc vs. Doc/MNTX). Drug administration was started 7 days after the inoculation of 60As6-Luc cells. Mice were treated with Doc or a combination of Doc and MNTX 2 times a week until the endpoint criteria were met. B, visceral pain-related behavior of peritoneal metastasis model mice. Visceral pain-related behavior was assessed in terms of the degree of hunching and the time spent hunching before each drug treatment at 35 days after the inoculation of 60As6-Luc cells (mean ± SD, n = 14 each, *<i>p</i><0.05). C, survival curves of peritoneal metastasis mice of <i>OGFR</i>-shRNA transfected 60As6 cells (OGFR-KD) treated with saline, Doc, or Doc/MNTX (0.3 mg/kg) (n = 5, *<i>p</i><0.05, vs. saline, no significance in Doc vs. Doc/MNTX).</p

Blockade of OGF signaling by MNTX increased the growth of diffuse-type GC cells co-cultured with mesothelial cells.

<p>A, RT-PCR analyses of <i>Penk</i> and <i>Ogfr</i>, in mouse mesothelial cells (1Cs-mM). B, schematic illustration of the system for co-culture of 60As6-GFP and 1Cs-mM. C, Growth of 60As6-GFP cells co-cultured with 1Cs-mM cells in the presence or absence of MNTX (10^-5 M) for 72 h. Scale bar, 20 μm. D, the growth of 60As6-GFP cells was calculated (mean ± SD, n = 3 each, *<i>p</i><0.05). E, growth of the diffuse-type GC cell line 60As6 cells, the intestinal-type GC cell line HSC-42 cells, the pancreatic cancer cell line PANC-1 cells, and primary cultured GC cells derived from the ascites of a patient NSC-16C cells treated with Doc (10^-9 M) or a vehicle for 48 h, and subsequently treated with Doc, Doc/MNTX (10^-6 M) or a vehicle for 48 h. Cells were counted with a hemacytometer (mean ± SD, n = 4 each, *<i>p</i><0.05, vs. control, #<i>p</i><0.05, Doc vs. Doc/MNTX).</p

<i>PENK</i> encoding opioid growth factor (OGF) is preferentially expressed in diffuse-type gastric cancers (GCs).

<p>Representative histological image (hematoxylin-eosin, HE) and Ki-67 immunostaining of diffuse-type GC (A) and intestinal-type GC (B). Scale bar, 50 μm. C, supervised clustering analysis of 892 specifically expressed genes in 12 diffuse-type and 18 intestinal-type GCs. By the Wilcoxon u-test (<i>p</i><0.05) and a 2-fold change, 188 genes were selected as specific genes for 18 intestinal-type GCs, and 704 genes were selected as specific genes for 12 diffuse-type GCs. The results of a two-dimensional hierarchical clustering analysis of the 892 selected genes are shown. D, RT-PCR analyses of OGF signaling molecules, <i>PENK</i> and its receptor <i>OGFR</i>, in diffuse-type and intestinal-type GCs.</p

Mouse models of intraperitoneal low-dose Doc therapy corresponding to 3 different phases (early, middle, and late) in the progression of peritoneal dissemination.

<p>Survival curves for the early phase (A), middle phase (B), and late phase (C) of a peritoneal metastasis model. Administration of Doc (0.5 mg/kg) was started 1 day (A), 7 days (B) or 14 days (C) after the inoculation of 60As6-Luc cells, and was continued until the endpoint criteria were reached (n = 5, *<i>p</i><0.05, vs. saline). D, representative histological image (hematoxylin-eosin, HE) and Ki-67 immunostaining of 60As6 xenograft. Scale bar, 50 μm. E, detection of the progression of peritoneal dissemination in real-time using an <i>in vivo</i> photon-counting analysis of mice treated with saline, Doc or Doc/MNTX (0.3 mg/kg). Beginning on day 7 after inoculation, the mice were divided into 4 groups based on photon counts. The mice were then treated intraperitoneally with the above reagents twice weekly until the endpoint criteria were met (middle phase).</p