Ebola Virus Localization in the Macaque Reproductive Tract during Acute Ebola Virus Disease
2018; Elsevier BV; Volume: 188; Issue: 3 Linguagem: Inglês
10.1016/j.ajpath.2017.11.004
ISSN1525-2191
AutoresDonna L. Perry, Louis Huzella, John G. Bernbaum, Michael R. Holbrook, Peter B. Jahrling, Katie R. Hagen, Matthias J. Schnell, Reed F. Johnson,
Tópico(s)Viral Infections and Vectors
ResumoSexual transmission of Ebola virus (EBOV) has been demonstrated more than a year after recovery from the acute phase of Ebola virus disease (EVD). The mechanisms underlying EBOV persistence and sexual transmission are not currently understood. Using the acute macaque model of EVD, we hypothesized EBOV would infect the reproductive tissues and sought to localize the infection in these tissues using immunohistochemistry and transmission electron microscopy. In four female and eight male macaques that succumbed to EVD between 6 and 9 days after EBOV challenge, we demonstrate widespread EBOV infection of the interstitial tissues and endothelium in the ovary, uterus, testis, seminal vesicle, epididymis, and prostate gland, with minimal associated tissue immune response or organ pathology. Given the widespread involvement of EBOV in the reproductive tracts of both male and female macaques, it is reasonable to surmise that our understanding of the mechanisms underlying sexual transmission of EVD and persistence of EBOV in immune-privileged sites would be facilitated by the development of a nonhuman primate model in which the macaques survived past the acute stage into convalescence. Sexual transmission of Ebola virus (EBOV) has been demonstrated more than a year after recovery from the acute phase of Ebola virus disease (EVD). The mechanisms underlying EBOV persistence and sexual transmission are not currently understood. Using the acute macaque model of EVD, we hypothesized EBOV would infect the reproductive tissues and sought to localize the infection in these tissues using immunohistochemistry and transmission electron microscopy. In four female and eight male macaques that succumbed to EVD between 6 and 9 days after EBOV challenge, we demonstrate widespread EBOV infection of the interstitial tissues and endothelium in the ovary, uterus, testis, seminal vesicle, epididymis, and prostate gland, with minimal associated tissue immune response or organ pathology. Given the widespread involvement of EBOV in the reproductive tracts of both male and female macaques, it is reasonable to surmise that our understanding of the mechanisms underlying sexual transmission of EVD and persistence of EBOV in immune-privileged sites would be facilitated by the development of a nonhuman primate model in which the macaques survived past the acute stage into convalescence. Sexual transmission of filoviruses has been suspected for as long as these viruses have been recognized as human pathogens. During the first recorded outbreak of Marburg virus disease in 1967, sexual transmission from an infected man to a woman was presumed but never proved.1Martini G.A. Marburg virus disease.Postgrad Med J. 1973; 49: 542-546Crossref PubMed Scopus (56) Google Scholar Ebola virus (EBOV) was detected in the semen of a researcher infected while handling diagnostic samples from the first recorded EBOV outbreak in 1976.2Emond R.T. Evans B. Bowen E.T. Lloyd G. A case of Ebola virus infection.Br Med J. 1977; 2: 541-544Crossref PubMed Scopus (262) Google Scholar The 2014 to 2016 EBOV outbreak in West Africa again raised the question of sexual transmission of filoviruses and the potential for asymptomatic infections and EBOV persistence in immune-privileged sites.3Glynn J.R. Bower H. Johnson S. Houlihan C.F. Montesano C. Scott J.T. Semple M.G. Bangura M.S. Kamara A.J. Kamara O. Mansaray S.H. Sesay D. Turay C. Dicks S. Wadoum R.E.G. Colizzi V. Checchi F. Samuel D. Tedder R.S. Asymptomatic infection and unrecognised Ebola virus disease in Ebola-affected households in Sierra Leone: a cross-sectional study using a new non-invasive assay for antibodies to Ebola virus.Lancet Infect Dis. 2017; 17: 645-653Abstract Full Text Full Text PDF PubMed Scopus (71) Google Scholar, 4Jacobs M. Rodger A. Bell D.J. Bhagani S. Cropley I. Filipe A. et al.Late Ebola virus relapse causing meningoencephalitis: a case report.Lancet. 2016; 388: 498-503Abstract Full Text Full Text PDF PubMed Scopus (230) Google Scholar, 5Sow M.S. Etard J.F. Baize S. Magassouba N.F. Faye O. Msellati P. et al.New evidence of long-lasting persistence of Ebola virus genetic material in semen of survivors.J Infect Dis. 2016; 214: 1475-1476Crossref PubMed Scopus (63) Google Scholar, 6Varkey J.B. Shantha J.G. Crozier I. Kraft C.S. Lyon G.M. Mehta A.K. Kumar G. Smith J.R. Kainulainen M.H. Whitmer S. Stroher U. Uyeki T.M. Ribner B.S. Yeh S. Persistence of Ebola virus in ocular fluid during convalescence.N Engl J Med. 2015; 372: 2423-2427Crossref PubMed Scopus (325) Google Scholar Findings from >17,000 survivors of the outbreak in West Africa suggest sexual transmission is rare. To date, only two recorded incidences of sexual transmission of EBOV from that outbreak have been documented.7Diallo B. Sissoko D. Loman N.J. Bah H.A. Bah H. Worrell M.C. Conde L.S. Sacko R. Mesfin S. Loua A. Kalonda J.K. Erondu N.A. Dahl B.A. Handrick S. Goodfellow I. Meredith L.W. Cotten M. Jah U. Guetiya Wadoum R.E. Rollin P. Magassouba N. Malvy D. Anglaret X. Carroll M.W. Aylward R.B. Djingarey M.H. Diarra A. Formenty P. Keita S. Gunther S. Rambaut A. Duraffour S. Resurgence of Ebola virus disease in Guinea linked to a survivor with virus persistence in seminal fluid for more than 500 days.Clin Infect Dis. 2016; 63: 1353-1356Crossref PubMed Scopus (146) Google Scholar, 8Mate S.E. Kugelman J.R. Nyenswah T.G. Ladner J.T. Wiley M.R. Cordier-Lassalle T. et al.Molecular evidence of sexual transmission of Ebola virus.N Engl J Med. 2015; 373: 2448-2454Crossref PubMed Scopus (309) Google Scholar However, the implications of EBOV transmission by this route are significant given an Ebola virus disease (EVD) mortality rate of >40%.9Crozier I. Ebola virus RNA in the semen of male survivors of Ebola virus disease: the uncertain gravitas of a privileged persistence.J Infect Dis. 2016; 214: 1467-1469Crossref PubMed Scopus (16) Google Scholar, 10Kuhn J.H. Bavari S. Asymptomatic Ebola virus infections: myth or reality?.Lancet Infect Dis. 2017; 17: 570-571Abstract Full Text Full Text PDF PubMed Scopus (10) Google Scholar We hypothesized that EBOV would infect the reproductive tissues in the macaque model of acute EVD. The purpose of this study was to identify and localize the virus within the reproductive tissues in the macaque model, typically acutely fatal between 6 and 10 days after i.m. challenge. Using this EVD model, we demonstrate EBOV infection of the interstitial or supporting connective tissues of the male and female reproductive organs, with minimal associated tissue immune response or organ pathology. Twelve macaques, seven rhesus (Macaca mulatta; one female and six males) and five cynomolgus (Macaca fascicularis; three females and two males), ranging in age from 35 to 58 months, were challenged with 1000 plaque-forming units i.m. of EBOV Makona C05.11Baize S. Pannetier D. Oestereich L. Rieger T. Koivogui L. Magassouba N.F. Soropogui B. Sow M.S. Keïta S. De Clerck H. Tiffany A. Dominguez G. Loua M. Traoré A. Kolié M. Malano E.R. Heleze E. Bocquin A. Mély S. Raoul H. Caro V. Cadar D. Gabriel M. Pahlmann M. Tappe D. Schmidt-Chanasit J. Impouma B. Diallo A.K. Formenty P. Van Herp M. Günther S. Emergence of Zaire Ebola virus disease in Guinea.N Engl J Med. 2014; 371: 1418-1425Crossref PubMed Scopus (1025) Google Scholar Macaques were euthanized after meeting end point criteria between 6 and 9 days after EBOV challenge. Each macaque underwent a complete postmortem examination when predetermined end point criteria12Warren T.K. Trefry J.C. Marko S.T. Chance T.B. Wells J.B. Pratt W.D. Johnson J.C. Mucker E.M. Norris S.L. Chappell M. Dye J.M. Honko A.N. Euthanasia assessment in ebola virus infected nonhuman primates.Viruses. 2014; 6: 4666-4682Crossref PubMed Scopus (19) Google Scholar for EVD were reached. Reproductive tissues were collected from all macaques for routine histology, immunohistochemistry (IHC) for EBOV viral protein 40 (VP40) matrix protein and/or glycoprotein (GP), and transmission electron microscopy examination.13Noda T. Ebihara H. Muramoto Y. Fujii K. Takada A. Sagara H. Kim J.H. Kida H. Feldmann H. Kawaoka Y. Assembly and budding of Ebolavirus.PLoS Pathog. 2006; 2: e99Crossref PubMed Scopus (133) Google Scholar Immunohistochemistry for EBOV VP40 and/or GP was positive in the reproductive organs of all 12 macaques. Transmission electron microscopy of the reproductive tissues was performed in 11 of 12 macaques that succumbed to EVD, and widespread EBOV infection of the stromal connective tissues, including endothelial cells, was observed in all macaques examined. A summation of findings can be found in Table 1.Table 1Signalment, EBOV in Peripheral Blood, and EBOV Distribution in the Reproductive Tract of Female and Male MacaquesAnimal IDMacaque speciesAge, monthsNecropsy after inoculation, daysEBOV vRNA, copy/mL (log10)EBOV IHC resultsTEM resultsOvaryUterusTestisProstate glandSeminal vesicleEpididymis1Cynomolgus46710.6Stromal/vascularStromal/vascularStromal/EC2Cynomolgus5389.96Stromal/vascularStromal/vascularStromal3Cynomolgus53710.1Stromal/vascularStromal/vascularStromal/EC4Rhesus35710.4Stromal/vascularStromal/vascularStromal5Cynomolgus48610.3Stromal/vascularStromal/vascularStromal/vascularStromal/vascularStromal/EC6Cynomolgus44810Stromal/vascularStromal/vascularStromal/vascularStromal/vascularStromal/EC7Rhesus4498.83Stromal/vascularStromal/vascularStromal/vascularNPStromal/EC8Rhesus4879.78Stromal/vascularStromal/vascularStromal/vascularNPStromal/EC9Rhesus5889.95Stromal/vascularStromal/vascularStromal/vascularStromal/vascularStromal/EC10Rhesus56710.2Stromal/vascularStromal/vascularStromal/vascularStromal/vascularStromal/EC11Rhesus35710.1Stromal/vascularStromal/vascularStromal/vascularStromal/vascularStromal/EC12Rhesus38610.6Stromal/vascularStromal/vascularStromal/vascularStromal/vascularNPEBOV, Ebola virus; EC, endothelial cell; ID, identification; IHC, immunohistochemistry; NP, not performed; TEM, transmission electron microscopy; vRNA, viral RNA. Open table in a new tab EBOV, Ebola virus; EC, endothelial cell; ID, identification; IHC, immunohistochemistry; NP, not performed; TEM, transmission electron microscopy; vRNA, viral RNA. This study was performed in strict adherence to the Guide for the Care and Use of Laboratory Animals14Committee for the Update of the Guide for the Care and Use of Laboratory Animals National Research Council: Guide for the Care and Use of Laboratory Animals.Eighth Edition. National Academies Press, Washington, DC2011Crossref Google Scholar of the NIH, the Office of Animal Welfare, and the US Department of Agriculture. All work was approved by the US National Institute of Allergy and Infectious Diseases, Division of Clinical Research Animal Care and Use Committee, and performed at the US National Institute of Allergy and Infectious Diseases Research Facilities. Procedures were performed after animals had been anesthetized by trained personnel under the supervision of veterinary staff. Food and water were available ad libitum. This study includes 12 macaques that served as controls in three separate studies that were designed to evaluate the efficacy of a therapeutic agent intended to protect against the development of EVD. The first two experiments are described by Johnson et al.15Johnson R.F. Kurup D. Hagen K.R. Fisher C. Keshwara R. Papaneri A. Perry D.L. Cooper K. Jahrling P.B. Wang J.T. ter Meulen J. Wirblich C. Schnell M.J. An inactivated Rabies virus–based Ebola vaccine, FILORAB1, adjuvanted with glucopyranosyl lipid A in stable emulsion confers complete protection in nonhuman primate challenge models.J Infect Dis. 2016; 214: S342-S354Crossref PubMed Scopus (23) Google Scholar The seven rhesus macaques (M. mulatta) and five cynomolgus macaques (M. fascicularis) ranged in age from 35 to 58 months, with a total of four females (three cynomolgus and one rhesus) and eight males (two cynomolgus and six rhesus). These 12 macaques were randomized to control groups before EBOV i.m. challenge with EBOV (Zaire species) in the lateral head of the right triceps muscle using the Makona C05 EBOV isolate at a target dose of 1000 plaque-forming units.11Baize S. Pannetier D. Oestereich L. Rieger T. Koivogui L. Magassouba N.F. Soropogui B. Sow M.S. Keïta S. De Clerck H. Tiffany A. Dominguez G. Loua M. Traoré A. Kolié M. Malano E.R. Heleze E. Bocquin A. Mély S. Raoul H. Caro V. Cadar D. Gabriel M. Pahlmann M. Tappe D. Schmidt-Chanasit J. Impouma B. Diallo A.K. Formenty P. Van Herp M. Günther S. Emergence of Zaire Ebola virus disease in Guinea.N Engl J Med. 2014; 371: 1418-1425Crossref PubMed Scopus (1025) Google Scholar All macaques succumbed to EVD between 6 and 9 days after EBOV challenge. Nine pre-EBOV challenge blood draws were performed in each macaque, the last at 15 days before EBOV challenge (0 day). After EBOV challenge, blood draws were performed every other day starting at 2 days until 8 days after EBOV challenge. The last blood draw was performed immediately before necropsy. Complete blood cell counts, select serum chemistries, and real-time quantitative PCR for viremia were performed on these samples. Whole blood was inactivated in TRIzol LS (Thermo Fisher Scientific, Waltham, MA) in accordance with established methods for inactivation of risk group 4 pathogens. Briefly, total RNA was isolated using the QIAamp Viral RNA Mini Kit (Qiagen, Germantown, MD) using 700 μL of TRIzol LS inactivated sample that was added to 280 μL of Qiagen Buffer AVL containing carrier RNA. The sample was eluted in 70 μL of Buffer AVE, aliquoted, and frozen until assayed. Whole blood viral load was measured using BEI Resources Critical Reagents Program (Manassas, VA) EZ1 quantitative RT-PCR kit assay, in accordance with manufacturer's instructions, and reported as viral RNA copies (log10) per mL of sample. Reproductive tissue collected from females (uterus and ovaries) and males (testes, prostate, seminal vesicles, head, and tail of the epididymides) at necropsy was fixed in 10% neutral-buffered formalin in preparation for routine histopathology and immunohistochemistry. Ebola virus immunohistochemistry was performed on routinely processed tissue with an anti-EBOV VP40 (catalog number 0201-016; IBT Bioservices, Rockville, MD) or anti-EBOV GP antibody (catalog number 0301-015; IBT Bioservices), followed by a biotinylated anti-mouse (catalog number 115-065-166; Jackson Immunoresearch Laboratories, Westgrove, PA; for VP40) or anti-rabbit (catalog number 111-065-144; Jackson Immunoresearch Laboratories; for GP) secondary antibody and an avidin-biotin peroxidase tertiary antibody (catalog number PK-6100; Vector Laboratories, Burlingame, CA). Ebola virus was visualized with 3,3′-diaminobenzidine chromogen (catalog number BDB2004L; Biocare, Pacheco, CA), counterstained with hematoxylin, and assessed by a single pathologist (D.L.P.). Immunohistochemical controls included Ebola virus–infected liver from an EBOV-infected macaque and liver from an EBOV-naïve macaque, as positive and negative controls, respectively. In addition, assay controls (omission of the primary antibody) and isotype controls were performed for EBOV-VP40 (mouse IgG1; catalog number ab18443; Abcam, Cambridge, MA) and EBOV-GP (rabbit IgG; catalog number ab27478; Abcam). The distribution of EBOV IHC staining in the reproductive tissues was similar with anti-EBOV VP40 and anti-EBOV GP. For conventional thin-section microscopic evaluation, tissues were fixed for 72 hours in 2.5% glutaraldehyde and 2.0% paraformaldehyde (E.M. Sciences, Warrington, PA) in Millonig's sodium phosphate buffer (Tousimis Research, Rockville, MD). Fixed tissues were washed repeatedly in Millonig's buffer and then incubated for 2 hours in 1.0% osmium tetroxide. After rinsing steps in ultrapure water and en bloc staining with 2.0% uranyl acetate, tissues were dehydrated in a series of graded ethanols and infiltrated and embedded in Spurr's plastic resin (E.M. Sciences). Embedded blocks were divided into sections using a Leica UC7 ultramicrotome (Leica, Wetzlar, Germany). Sections (70 to 80 nm thick) were collected on 200 mesh copper grids and poststained with Reynold's lead citrate. Samples were examined in an FEI Tecnai Spirit Twin transmission electron microscope (FEI Company, Hillsboro, OR), operating at 80 kV. Histopathological lesions in the ovary secondary to EVD were not observed in the macaques examined. Inclusion bodies could be seen in the mesenchymal thecal cells surrounding secondary and tertiary ovarian follicles. Immunohistochemical staining for EBOV GP in the ovary was multifocally positive in the thecal cells surrounding secondary and tertiary ovarian follicles and in the vascular endothelium in macaques that succumbed to EVD (Figure 1). Immunohistochemical positivity in the granulosa cells was rare. Ultrastructural examination of the ovary confirmed viral infection of ovarian stromal cells and endothelial cells (Figure 1). Fimbrial epithelial cells of the salpinx (Fallopian tube or oviduct) stained positive multifocally for EBOV VP40 and GP (data not shown). Histopathological lesions in the uterus secondary to EVD were not observed in the macaques examined. Immunohistochemical staining for EBOV VP40 revealed widespread positivity in the vasculature, endometrial stromal cells, and smooth muscle cells of the myometrium in macaques that succumbed to EVD (Figure 1). Ultrastructural examination of the uterus confirmed viral infection of endometrial stromal cells and smooth muscles cells of the myometrium (Figure 1). Histopathological lesions in the testis were uncommon but included the presence of spermatid giant cells and oligospermia; however, macaque species are seasonal breeders and sperm density must be interpreted in the context of age, social rank, recent changes in social housing,16Niehoff M.O. Bergmann M. Weinbauer G.F. Effects of social housing of sexually mature male cynomolgus monkeys during general and reproductive toxicity evaluation.Reprod Toxicol. 2010; 29: 57-67Crossref PubMed Scopus (20) Google Scholar and photoperiod or season.17Zamboni L. Conaway C.H. van Pelt L. Seasonal changes in production of semen in free-ranging Rhesus monkeys.Biol Reprod. 1974; 11: 251-267Crossref PubMed Scopus (47) Google Scholar Uncommonly, thrombosis with infarction of testicular stroma occurred secondary to EVD-induced coagulopathy, resulting in areas of ischemic necrosis of the testicular tissue. Immunohistochemistry for EBOV VP40 and GP in the testis revealed widespread positivity in the interstitial connective tissues, including endothelial cells (Figure 2). Ultrastructural examination of the testis confirmed viral infection of interstitial connective tissues, including endothelial cells (Figure 2). In the prostate gland and seminal vesicle, histopathological lesions secondary to EVD were not observed, despite widespread immunohistochemical positivity for EBOV VP40 and GP in the stromal connective tissues (Figures 2 and 3). Epithelial cell positivity for EBOV by IHC in these organs was rare. In the head and tail of the epididymis, histopathological lesions secondary to EVD were nonspecific, but included interstitial edema and, rarely, vascular thrombosis. Similar widespread multifocal positivity for EBOV VP40 and GP was detected in the interstitial connective tissue supporting the tubular epithelium of the epididymis in acutely EVD-affected macaques (Figure 3). Ultrastructural examination of the prostate gland, epididymis, and seminal vesicle confirmed viral infection of interstitial mesenchymal cells, including endothelial cells (Figures 2 and 3). Mature EBOV particles were seen within the disrupted membranes of an expanded endoplasmic reticulum; however, the virus was only observed to bud from the cell surface or plasma membrane. Ebola virus GP is known to accumulate in the endoplasmic reticulum of infected cells,18Bhattacharyya S. Hope T.J. Full-length Ebola glycoprotein accumulates in the endoplasmic reticulum.Virol J. 2011; 8: 11Crossref PubMed Scopus (25) Google Scholar, 19Alazard-Dany N. Volchkova V. Reynard O. Carbonnelle C. Dolnik O. Ottmann M. Khromykh A. Volchkov V.E. Ebola virus glycoprotein GP is not cytotoxic when expressed constitutively at a moderate level.J Gen Virol. 2006; 87: 1247-1257Crossref PubMed Scopus (64) Google Scholar which may partially explain the marked expansion of endoplasmic reticulum membranes observed occasionally in EBOV-infected cells. Within the ductus deferens, epithelial positivity for EBOV VP40 protein was observed (data not shown). Using the macaque model of acute EVD, we have demonstrated early and widespread infection of the male and female reproductive tract after i.m. EBOV challenge. Ebola virus replication occurs predominantly within the mesenchymal or supporting stromal cells of the reproductive tract. The presence of the virus in the ovary and uterus in the macaque model of EVD has not been reported previously. However, detection of EBOV in the thecal mesenchymal cells surrounding ovarian follicles and IHC positivity associated with inflammation in necrosis in the uterus have been demonstrated in the guinea pig model of EVD.20Connolly B.M. Steele K.E. Davis K.J. Geisbert T.W. Kell W.M. Jaax N.K. Jahrling P.B. Pathogenesis of experimental Ebola virus infection in guinea pigs.J Infect Dis. 1999; 179: S203-S217Crossref PubMed Scopus (262) Google Scholar The effect of EBOV infection of thecal cells on the denouement of secondary and tertiary ovarian follicles in macaques is unknown. The effect of EBOV infection of smooth muscle cells in the uterus is also unknown; however, in pregnant women with EVD, an average maternal death rate of 82% and a fetal death rate of 100% have been reported.21Muehlenbachs A. de la Rosa Vázquez O. Bausch D.G. Schafer I.J. Paddock C.D. Nyakio J.P. Lame P. Bergeron E. McCollum A.M. Goldsmith C.S. Bollweg B.C. Prieto M.A. Lushima R.S. Ilunga B.K. Nichol S.T. Shieh W.-J. Ströher U. Rollin P.E. Zaki S.R. Ebola virus disease in pregnancy: clinical, histopathologic, and immunohistochemical findings.J Infect Dis. 2017; 215: 64-69Crossref PubMed Scopus (36) Google Scholar Ebola virus is able to infect the fetus.22Black B.O. Caluwaerts S. Achar J. Ebola viral disease and pregnancy.Obstet Med. 2015; 8: 108-113Crossref PubMed Scopus (42) Google Scholar In the placenta, fetal-origin syncytiotrophoblasts can be infected with the Sudan and Bundibugyo viruses.21Muehlenbachs A. de la Rosa Vázquez O. Bausch D.G. Schafer I.J. Paddock C.D. Nyakio J.P. Lame P. Bergeron E. McCollum A.M. Goldsmith C.S. Bollweg B.C. Prieto M.A. Lushima R.S. Ilunga B.K. Nichol S.T. Shieh W.-J. Ströher U. Rollin P.E. Zaki S.R. Ebola virus disease in pregnancy: clinical, histopathologic, and immunohistochemical findings.J Infect Dis. 2017; 215: 64-69Crossref PubMed Scopus (36) Google Scholar The only known congenitally infected infant to survive EBOV infection was treated on 2, 5, 8, and 11 days of life with the monoclonal antibody cocktail, ZMapp, and received an i.v. transfusion of leukocytes from an EBOV survivor on day 11 of life; beginning on day 19 of life, this infant was treated for 12 days with the nucleotide analog prodrug, GS-5734.23Dornemann J. Burzio C. Ronsse A. Sprecher A. De Clerck H. Van Herp M. Kolie M.C. Yosifiva V. Caluwaerts S. McElroy A.K. Antierens A. First newborn baby to receive experimental therapies survives Ebola virus disease.J Infect Dis. 2017; 215: 171-174PubMed Google Scholar Ebola virus is shed in breast milk, and epidemiologically linked transmission from an asymptomatic mother to a 9-month-old child through breast milk has been reported.24Sissoko D. Keita M. Diallo B. Aliabadi N. Fitter D.L. Dahl B.A. Akoi Bore J. Raymond Koundouno F. Singethan K. Meisel S. Enkirch T. Mazzarelli A. Amburgey V. Faye O. Alpha Sall A. Magassouba N. Carroll M.W. Anglaret X. Malvy D. Formenty P. Bruce Aylward R. Keita S. Harouna Djingarey M. Loman N.J. Gunther S. Duraffour S. Ebola virus persistence in breast milk after no reported illness: a likely source of virus transmission from mother to child.Clin Infect Dis. 2017; 64: 513-516PubMed Google Scholar The presence or absence of EBOV persistence in women is understudied, as are the effects of EVD in pregnant women and their offspring. In men, temporal evidence and sequence analysis of EBOV samples from the 2014 to 2016 West Africa outbreak demonstrated sexual transmission of EBOV to women from 6 months to >1 year after recovery from EVD.7Diallo B. Sissoko D. Loman N.J. Bah H.A. Bah H. Worrell M.C. Conde L.S. Sacko R. Mesfin S. Loua A. Kalonda J.K. Erondu N.A. Dahl B.A. Handrick S. Goodfellow I. Meredith L.W. Cotten M. Jah U. Guetiya Wadoum R.E. Rollin P. Magassouba N. Malvy D. Anglaret X. Carroll M.W. Aylward R.B. Djingarey M.H. Diarra A. Formenty P. Keita S. Gunther S. Rambaut A. Duraffour S. Resurgence of Ebola virus disease in Guinea linked to a survivor with virus persistence in seminal fluid for more than 500 days.Clin Infect Dis. 2016; 63: 1353-1356Crossref PubMed Scopus (146) Google Scholar, 8Mate S.E. Kugelman J.R. Nyenswah T.G. Ladner J.T. Wiley M.R. Cordier-Lassalle T. et al.Molecular evidence of sexual transmission of Ebola virus.N Engl J Med. 2015; 373: 2448-2454Crossref PubMed Scopus (309) Google Scholar A recent report from Fischer et al25Fischer W.A. Brown J. Wohl D.A. Loftis A.J. Tozay S. Reeves E. Pewu K. Gorvego G. Quellie S. Cunningham C.K. Merenbloom C. Napravnik S. Dube K. Adjasoo D. Jones E. Bonarwolo K. Hoover D. Ebola virus ribonucleic acid detection in semen more than two years after resolution of acute Ebola virus infection.Open Forum Infect Dis. 2017; 4 (ofx155-ofx)Crossref Google Scholar described the longest interval, 965 days, between onset of EVD and the detection of EBOV RNA in semen. The prevalence of detection was significantly higher in older men (median age, 41.8 years), and detection was intermittent. On the basis of our findings, we hypothesize that persistence is established in the interstitial tissues of the reproductive tract and tissue macrophages are the route by which EBOV is transmitted from stromal replication sites in the seminal vesicle, epididymis, prostate gland, and testis into the seminal fluid. Because this study used tissue collected adjunctively at necropsy from ongoing studies, the collection and examination of seminal fluid was not possible, and no fresh tissue was collected for RNA sequencing. Infection of monocytes and macrophages facilitates systemic spread of the EBOV but neutrophils and B, T, and natural killer cells, critical for both the innate and humoral immune response, are not infected.26Wang H. Shi Y. Song J. Qi J. Lu G. Yan J. Gao George F. Ebola viral glycoprotein bound to its endosomal receptor Niemann-Pick C1.Cell. 2016; 164: 258-268Abstract Full Text Full Text PDF PubMed Scopus (169) Google Scholar Although we have demonstrated active EBOV infection of endothelial cells in reproductive tissues, endothelial cells exhibit a high degree of heterogeneity, and endothelial cell infection within one tissue type likely does not translate to permissivity of viral infection in another.27Potente M. Makinen T. Vascular heterogeneity and specialization in development and disease.Nat Rev Mol Cell Biol. 2017; 18: 477-494Crossref PubMed Scopus (277) Google Scholar Although the macaque model of human EVD is thought to have a high fidelity, it is unknown if the distribution of the virus is similar in the reproductive tract of affected humans or why sexual transmission in convalescent human populations is rare. Martines et al28Martines R.B. Ng D.L. Greer P.W. Rollin P.E. Zaki S.R. Tissue and cellular tropism, pathology and pathogenesis of Ebola and Marburg viruses.J Pathol. 2015; 235: 153-174Crossref PubMed Scopus (204) Google Scholar reported positivity for EBOV antigens by IHC in testicular endothelium and focally within the seminiferous tubular cells in one man. Zeng et al29Zeng X. Blancett C.D. Koistinen K.A. Schellhase C.W. Bearss J.J. Radoshitzky S.R. Honnold S.P. Chance T.B. Warren T.K. Froude J.W. Cashman K.A. Dye J.M. Bavari S. Palacios G. Kuhn J.H. Sun M.G. Identification and pathological characterization of persistent asymptomatic Ebola virus infection in rhesus monkeys.Nat Microbiol. 2017; 2: 17113Crossref PubMed Scopus (81) Google Scholar recently reported detection of EBOV viral RNA in the interstitial tissues of the testis and epididymis, in the same pattern we describe herein, at day 43 after EBOV exposure in 1 of 76 nonhuman primate EVD survivors after experimental countermeasure treatment. These findings support the need for an established definition of EBOV persistence in the macaque model of EVD and to determine whether the presence of viral RNA in the semen equates to the presence of infectious EBOV. The findings from Fischer et al25Fischer W.A. Brown J. Wohl D.A. Loftis A.J. Tozay S. Reeves E. Pewu K. Gorvego G. Quellie S. Cunningham C.K. Merenbloom C. Napravnik S. Dube K. Adjasoo D. Jones E. Bonarwolo K. Hoover D. Ebola virus ribonucleic acid detection in semen more than two years after resolution of acute Ebola virus infection.Open Forum Infect Dis. 2017; 4 (ofx155-ofx)Crossref Google Scholar and Zeng et al29Zeng X. Blancett C.D. Koistinen K.A. Schellhase C.W. Bearss J.J. Radoshitzky S.R. Honnold S.P. Chance T.B. Warren T.K. Froude J.W. Cashman K.A. Dye J.M. Bavari S. Palacios G. Kuhn J.H. Sun M.G. Identification and pathological characterization of persistent asymptomatic Ebola virus infection in rhesus monkeys.Nat Microbiol. 2017; 2: 17113Crossref PubMed Scopus (81) Google Scholar also highlight the need to evaluate multiple seminal samples from a diverse study cohort for the presence of EBOV to determine whether age affects the incidence of EBOV persistence. Proposed EVD countermeasures need to be evaluated for efficacy and to determine whether they facilitate the development of EBOV persistence. Several RNA viruses that establish persistence in infected hosts may provide valuable insight into EBOV persistence.30Randall R.E. Griffin D.E. Within host RNA virus persistence: mechanisms and consequences.Curr Opin Virol. 2017; 23: 35-42Crossref PubMed Scopus (55) Google Scholar Equine arteritis virus establishes persistent infection in stallions after recovery from clinical disease. The stromal cells of the ampulla, infiltrating tissue macrophages, T cells, and B cells in stallions are persistently infected, in the presence of neutralizing antibody.31Carossino M. Loynachan A.T. Canisso I.F. Cook R.F. Campos J.R. Nam B. Go Y.Y. Squires E.L. Troedsson M.H.T. Swerczek T. Del Piero F. Bailey E. Timoney P.J. Balasuriya U.B.R. Equine arteritis virus has specific tropism for stromal cells and CD8+ T and CD21+ B lymphocytes but not for glandular epithelium at the primary site of persistent infection in the stallion reproductive tract.J Virol. 2017; 91: e00418-17Crossref PubMed Scopus (18) Google Scholar Persistence of equine arteritis virus is associated with polymorphisms in the stallion's CXCL16 gene. Virus shedding in seminal fluid continues for an average of 165 days after infection in the absence of viremia and clinical evidence of reproductive dysfunction. 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