Can the Cervix Not Opeing During Birth Cause the Baby to Suffocate
J Immunol. Author manuscript; available in PMC 2014 Sep 3.
Published in final edited form as:
PMCID: PMC4153356
NIHMSID: NIHMS479461
Viral infection of the pregnant neck predisposes to ascending bacterial infection
Karen Racicot
*Department of Obstetrics and Gynecology, Yale School of Medicine, New Haven, CT
Ingrid Cardenas
†Department of Obstetrics and Gynecology Tuffs University, Boston MA
Vera Wünsche
*Section of Obstetrics and Gynecology, Yale School of Medicine, New Haven, CT
Paulomi Aldo
*Department of Obstetrics and Gynecology, Yale School of Medicine, New Oasis, CT
Seth Guller
*Section of Obstetrics and Gynecology, Yale School of Medicine, New Haven, CT
Robert Means
‡Department of Pathology, Yale School of Medicine, New Haven, CT
Roberto Romero
§Perinatology Research Branch, Eunice Kennedy Shriver National Institute of Child Wellness and Human Development, NIH, DHHS, Detroit
Gil Mor
*Department of Obstetrics and Gynecology, Yale School of Medicine, New Oasis, CT
Abstruse
Preterm nascency is the major crusade of neonatal mortality and morbidity, and bacterial infections that ascend from the lower female reproductive tract (FRT) are the most common route of uterine infection leading to preterm birth. The uterus and growing fetus are protected from ascending infection by the neck, which controls and limits microbial access past the production of mucus, cytokines and anti-microbial peptides (AMPs). If this barrier is compromised, leaner may enter the uterine cavity leading to preterm nascency. Using a mouse model, we demonstrate, for the get-go fourth dimension, that viral infection of the cervix, during pregnancy, reduces the capacity of the FRT to prevent bacterial infection of the uterus. This is due to differences in susceptibility of the cervix to infection by virus during pregnancy and the associated changes in TLR and AMP expression and role. We advise that preterm labor is a polymicrobial disease, which requires a multifactorial arroyo for its prevention and treatment.
Introduction
Preterm birth is the major cause of neonatal mortality and morbidity worldwide, still the underlying etiologies remain poorly understood (ane, 2). Preterm labor is a syndrome diagnosed in the presence of increased uterine contractility, cervical ripening, and/or membrane rupture or activation, which may occur in response to multiple pathological processes(1, ii). Neonates born with a fetal inflammatory response are more probable to develop short- and long-term complications in a higher place those expected for the gestational historic period at birth (3–five).
Numerous studies suggest that intrauterine infection is an of import mechanism leading to preterm labor and may account for 40% of preterm births (half-dozen–eight). However, this number may be college because many infections are probable to exist subclinical and the pathogenesis is not detected due to the lack of sensitivity of conventional civilization techniques(9) (10). Furthermore, our agreement of the normal flora of the female reproductive tract (FRT) is limited, and we have limited knowledge of the mechanisms controlling pathogenic bacteria and their relationship with intrauterine infection and preterm labor (eleven, 12).
All women have microorganisms in the lower genital tract (vulva, vagina and neck), however about studies indicate that amniotic fluid is commonly sterile and does not contain microbial products such as endotoxin. During pregnancy, intrauterine infections begin in the decidua, extend to the amnion and chorion and finally achieve the amniotic cavity and the fetus (13). Bacteria proceeds access to gestational tissues through one of three major routes: by ascending into the uterus from the lower tract, descending into the uterus from the peritoneal cavity or via the maternal apportionment (14) (6). Bacterial infections that ascend from the lower FRT are the most common route of uterine infection, and it is not known why some women suffer such infections that threaten pregnancies and fetal survival (xv). In a salubrious pregnancy, the uterus and growing fetus are protected from ascending infection by the cervix (12, sixteen) (17). The neck has a unique role in the FRT in that it actively controls and limits microbial access past the production of mucus, inflammatory cytokines and anti-microbial peptides (AMP)(xviii) (17). In not-pregnant women, the cervical mucus is a viscous fluid in the endocervical canal; however afterward conception the endocervical canal develops a structure called the cervical mucus plug, which is an anatomical and immunological barrier against ascending infection(nineteen). Indeed, assay of the composition and antimicrobial action of the cervical mucus plug revealed the presence of AMPs with stiff anti-microbial action (20). Besides expressed in the cervical epithelia are the pattern recognition receptors such equally Toll like receptors (TLRs) capable of sensing the presence of microorganisms and eliciting an innate allowed response characterized by the production of cytokines and AMPs (21, 22) (23, 24). Collectively, the neck plays a key role in the protection against ascending intraamniotic infection. If the mucus plug is expelled or cervical length is short, the gamble of ascending uterine infection increases.
Herpesviruses are the most common cause of viral-related perinatal neurologic injury in the USA (25). Withal, herpes simplex viruses (HSV-1 and HSV-2) and cytomegalovirus (CMV) (26) are among the eight known human herpesviruses reported to induce agin pregnancy and neonatal outcomes and have been plant in the amnion, placenta and even the lower reproductive tract of significant women(27). Murine gammaherpesvirus 68 (Murid herpesvirus iv ({"type":"entrez-nucleotide","attrs":{"text":"NC_001826.two","term_id":"146261990","term_text":"NC_001826.two"}}NC_001826.2); MHV-68) is a gammaherpesvirus of rodents that shares significant genomic co-linearity with two man pathogens, Epstein-Barr virus (EBV) and Kaposi'south sarcoma-associated herpesvirus (KSHV) (28).
Viral survival depends on their capacity to disable host defenses, specially the innate immune organisation, found latency and secure mechanism for reactivation. One style in which viruses could undermine host immunity is through the manipulation of innate immune receptors such equally TLRs. Nosotros have previously reported the use of MHV68 every bit a murine model to determine whether a subclinical viral infection sensitized the female parent to other microorganisms and induced preterm nativity (29). Our published data suggested that leaner or virus alone were not plenty to evoke preterm labor, but the combination was a threat. HSV and CMV have latency periods and tin exist reactivated via TLR signaling (thirty), therefore information technology tin be postulated that they could affect significant women the way MHV68 affects pregnant mice in our model.
We take now tested the hypothesis that a viral infection reduces the ability of the pregnant cervix to protect against ascending bacterial infection. Hither we testify a dramatic divergence in the capacity of the cervix to forbid ascending intrauterine bacterial infection in non-pregnant and pregnant mice and furthermore, we demonstrate that viral infection compromises the nature of the innate allowed response of the pregnant cervix predisposing to ascending intrauterine infection. Our results may explicate the differential sensitivity observed in pregnant women to ascending bacterial infections.
Materials and Methods
Animals and treatments
C57BL/6 mice were obtained from the Jackson Laboratory (Bar Harbor, ME); developed mice (8–12 wks of historic period) with vaginal plugs were infected i.p. at embryonic solar day 8.five post-formulation with either 1×x6 PFU MHV68 in 200 ul or DMEM (vehicle). To develop the ascending leaner model, E. coli (BL21) expressing RFP induced by IPTG and arabinose (pZS2, Addgene plasmid 26598, Michael Elowitz) were collected subsequently reaching an O.D.=.6, and resuspended gently in 40 uL of PBS. This was delivered in the vagina of mice sedated with isoflourane using a 200 uL gel tip and imaging was performed after 24hr using the Carestream In Vivo Imaging System FX PRO (Bruker Coorporation). Lymphoid aggregates were dissected from the stratum basalis afterwards gently removing the implantation site. For experiments determining gene expression and MHV68 titers in neck without hormone treatments, mice were sacrificed 7d post-infection (dpi) and organs were removed and stored at −lxxx°C. In experiments comparing non-pregnant and meaning mice, non-pregnant mice in diestrus were used. This was determined by morphology of the reproductive tract at time of sacrifice. For experiments determining the effect of systemic hormones, mice were ovariectomized, and after 21d treated with progesterone (500ug) and estrogen (500ng) or vehicle, south.c. for 3d. Both handling groups so received injections of MHV68 and continued to become hormone or vehicle every 2d for 7d. Cervix and spleen were then nerveless and MHV68 infection was determined past qPCR. All animals were maintained in the Yale University School of Medicine Animal Facility under specific pathogen-gratuitous conditions and all procedures reported in this manuscript were approved by the Yale University Institutional Animal Care and Utilize Commission. All in vivo experiments used betwixt 3 and half-dozen mice in at to the lowest degree two dissever independent experiments.
Mycoplasma
Ureaplasma urealyticum was purchased (27618) and reconstituted in ATCC media #2616, special modified formulation, as indicated by ATCC. Series dilutions of leaner were fabricated and incubated at 37C until medium changed color, indicating growth. At time of color change, individual tubes were stored at 4C until remaining dilutions exhibited growth. After 12h, bacteria were gently pelleted and resuspended in growth medium. A pocket-size aliquot was so used to determine colony-forming units (1×104/mL), while the remaining bacteria were injected intravaginally into mice at pregnancy E16.5 with or without MHV68 infection (MHV68 at d8.5).
Cell civilisation
Immortalized homo ectocervical cells (ECT1, ATCC, CRL-2614) were cultured in keratinocyte serum free medium (17005-042, Gibco, Grand Island, NY) with bovine pituitary excerpt and hEGF supplementation equally recommended by ATCC nether five% CO2 at 37°C. In blocking studies, 500 ug of Fibronectin (Gibco) was added to ECT1 cells for thirty min and removed. Cells were so infected with MHV68 for 30 min, washed and maintained in medium for 24 hours. To cake integrin blastoff three, the aforementioned protocol was used just with blocking antibodies for alpha 3 (P1B5, Millipore; all in vitro experiments were repeated 3 times.
MHV68 production and quantification
MHV68 expressing GFP was passaged in NIH 3T3 cells with DMEM plus 10% FBS. Later on lysis, supernatants were harvested, filtered (0.45 uM pore) and titered by 2-fold serial dilutions. To detect viral titers in mice, tissues were homogenized and approximately 25 mg of tissue from the reproductive tract or 10 mg of spleen were cut into small pieces and added to lysis buffer supplemented with proteinase K. Samples were incubated at 56C with shaking for 4–6 hours every bit recommended for the DNeasy claret and tissue kit (Qiagen, Valencia, CA). Cells from culture were lysed with the aforementioned buffer and vortexed at room temperature. All samples were and then processed co-ordinate to the DNeasy protocol. DNA concentration and purity was assessed using spectrophotometric analyses of 260/280 and 260/230 ratios. 100ng total DNA was then assayed using primers directed confronting MHV68 ORF53 and compared to a standard curve created using series dilutions of purified virus. Results are reported as copies per 100ng DNA.
RNA synthesis, cDNA synthesis and qPCR
RNA was extracted using the Trizol method (Invitrogen, Carlsbad, CA). RNA concentration and purity was assessed using spectrophotometric analyses of 260/280 ratios and but samples with values of one.7 or higher were used for PCR analysis. For quantitative analysis of mRNA, 1 ug of RNA was reverse transcribed for each sample using oligo (d)T priming and Verso cDNA kit which includes a DNAse enzyme (Invitrogen). Syber light-green main mix (KAPA Biosystems) and gene specific primers were added to the RT reactions that were diluted i:10 with nuclease gratis water and run on the CFX96, C1000 system qPCR machine (Biorad). No RT controls were used to confirm that values did non represent amplification of genomic DNA, and no template controls were used to confirm lack of contamination past whatever reagents. Values represented were normalized to beta actin and were calculated using the delta delta Ct method: delta delta Ct= delta ct treated- delta Ct command; results expressed as fold differences are 2ˆ-(average delta delta Ct) for negative delta delta Ct values or – (2ˆ[average delta delta Ct]) for positive delta delta Ct values.
Cytokines
Cytokine concentrations were adamant using cytokine multiplex assays from Bio-Rad. Briefly, wells were either loaded with 50 ul of prepared standard or 50 ul prison cell-free supernatant and incubated on an orbital shaker at 500 rpm for 2h in the night at RT. Wells were washed 3x with Bio-Rad wash reagent and samples were then incubated with 25 ul biotinylated detection Ab for 30 min, done, and incubated with 50 ul streptavidin-PE for 10 min. Afterwards final wash, samples were resuspended in assay buffer and measured using LUMINEX 200 (LUMINEX, Austin, TX). Cytokines included in this analysis are every bit follows: IL-Ib, IL-10, GM-CSF, IFNg, TNFa, IL-1a, IL-half dozen, IL-12p40, IL-12p70, One thousand-CSF, KC, MIP-1a, RANTES, MCP-i and MIP-1b.
Western blot analysis
Tissues were homogenized in phospho-jail cell lysis buffer (Cell Signaling, Danver, MA), and full protein concentrations were quantified using bicinchoninic acid (BCA) analysis (Pierce, Rockford, IL). Twenty micrograms of total proteins were dissolved in 1X sample buffer, boiled for 5 minutes and separated on a 12% SDS-Folio gel with 6% stacking gel in 1X electrode buffer at a abiding electric current of 70 mA for approximately ii 60 minutes. The proteins were transferred to nitrocellulose membranes (Protran, 0.2 μM, Schleicher & Schuell, Keene, NH) in a Mini-Protean II Prison cell apparatus (Bio-Rad Laboratories, Hercules, CA) at a constant 70 Five for 90 min with an ice pack. Not-fat milk (5%) was used equally a blocker (Fisher Scientific, Pittsburgh, PA), and immunoblotting was performed with a 1:500 dilution of primary antibodies in 2% NFM at 4°C overnight. Antibodies were Cell Signaling CS4749S (beta 1 integrin) and Millipore AB1920 (alpha iii integrin). Membranes were washed and a 1:10,000 dilution of caprine animal anti-rabbit or caprine animal anti-mouse IgG-horseradish peroxidase conjugate (Pierce) was added as appropriate. Membranes were washed and incubated with Western Lighting Plus (PerkinElmer, Waltham, MA) to find immunoreactive proteins.
Statistics
Differences between means (3 groups or more) were determined using analysis of variance and differences between two groups were analyzed using independent t-test functions of Graph pad inSTAT statistical software (La Jolla, CA). A p-value of ≤0.05 was considered significant and data is presented as mean ± standard error of the mean (SEM).
Results
Development of a murine model of ascending bacterial infection
Our kickoff objective was to determine whether a non-pathogenic class of East-coli could ascend through the FRT in pregnant and non-pregnant mice. Consequently, we inoculated genetically engineered leaner, E. coli expressing RFP (RFP-Due east. coli) into the vagina of healthy non-pregnant and significant mice and monitored their location using an imaging system. In not-pregnant animals, bacteria were clearly detected in the cervix and endometrial cavity within 24 hours (Fig. 1A). In dissimilarity, bacteria were not detectable in the cervix or uterine cavity of pregnant animals (Fig. 1B), indicating a dramatic resistance to microbial invasion of the uterine cavity during pregnancy. Bacteria were not observed at earlier time points in pregnant animals, suggesting there was no access, and non that the infection was there just rapidly eliminated (data non shown).
Murine model of ascending bacterial infection
Not-pregnant (A) and pregnant (B) mice were visualized 24 hours after receiving intravaginal injections of E. coli labeled with RFP. Legend indicates that blood-red colour in non-pregnant fauna has ascending bacterial infection in utero. NT=no bacterial injection, Bacteria=intravaginal bacterial injection; n=6. (C) Time course of murine model of ascending bacterial infection. Non-meaning mice were visualized 12, 24, 48 and 72 hours after receiving intravaginal injections of E. coli labeled with GFP. Bacteria are visualized in the vagina and cervix at 12h, found throughout the reproductive tract at 24 and 48 60 minutes, and are diminishing 72 hr post-infection.
To confirm the specificity of the signal and time course of ascending microbial invasion of the endometrial crenel, mice were inoculated in the vagina with the aforementioned E. coli but expressing GFP every bit the reporter gene. Animals were euthanized afterward 12, 24, 48 and 72 hours. Imaging of the genital tract was performed and as observed with RFP-E. coli, GFP- Due east. coli ascended through the uterus of the non-pregnant mice; furthermore, we observed an increase in fluorescent signal every bit a office of time (Fig 1C). That was non the instance in the FRT of meaning mice were there was no signal at whatever time (data not shown). These observations bespeak a dramatic deviation in the permissiveness of the not-significant and pregnant uterus to ascending infection from the lower genital tract.
Movement of Pathogenic Leaner through the mouse female reproductive tract
Since we institute that the pregnant FRT is capable of preventing an ascending E-coli bacterial infection, nosotros investigated whether this protection is operative with the bacteria virtually frequently found in the amniotic fluid of significant women with preterm labor, U. urealyticum (31, 32) (33). U. urealyticum was inoculated intravaginally on E15.v and after 24 hours decidua and lymphoid aggregates were harvested to determine if U. urealyticum was present in these tissues. Like as observed with E-coli, the pregnant FRT was able to prevent the migration of U. urealyticum towards the endometrial cavity (Fig 2B).
Ureaplasma urealyticum ascends into the uterus in MHV68 infected animals
Mice were infected with MHV68 or DMEM (control) at E8.5 of pregnancy, received an intravaginal injection of pathogenic U. urealyticum at E15.5, and were sacrificed (Sac) at E16.5 (A). NT= mice with no MHV68, MHV68= virus treated animals. Both groups received U. urealyticum; decidua and lymphoid aggregates are represented as fold difference from the same tissue from mice with no viral infection. Mice with MHV68 had higher concentrations of leaner in the decidua and lymphoid aggregates (Lymph Agg) compared to mice without viral infection (B). north=5
Since we observed that the normal FRT, during pregnancy, is highly protective of bacterial infection, we evaluated potential factors that would modify this protection and consequently would lead to an ascending bacterial infection every bit observed in pregnancy complications. Having previously established a mouse model of viral infection during pregnancy using a murine gammaherpes virus 68 (MHV68) which causes mice to be more susceptible to bacterial products (bacterial endotoxin or LPS),(15) we tested whether a systemic viral infection in pregnant animals could modify the resistance to microbial invasion of the uterine cavity. MHV68 was injected intra-peritoneal on E8.five of pregnancy and U. urealyticum was inoculated intravaginally on E15.v (Fig 2A). 24-hour interval later on bacterial inoculation nosotros harvested decidua and lymphoid aggregates to determine if U. urealyticum bacteria was present in these tissues as adamant using a specific PCR assay for U. urealyticum. U. urealyticum signal was significantly higher in the decidua and lymphoid aggregates in MHV68 infected mice compared to mice who had not been infected with MHV68 virus (Fig 2B) or a control grouping of pregnant animals not exposed to bacteria or virus (Information not shown). This data suggests that a viral infection during pregnancy alters the capacity of the FRT to control ascending bacterial infection.
Expression of antimicrobial peptides and TLR by the uterine cervix later viral infection with MHV68
The neck has a unique role functioning equally an interface betwixt the upper and lower FRT, providing protection to the uterine cavity confronting ascending intrauterine infection from the lower genital tract. During pregnancy epithelial cells of the cervix are responsible for the formation of the mucus plug that provides a mechanical and biochemical barrier to ascending infection (twenty). Since nosotros observed that a viral infection resulted in dramatic susceptibility to microbial invasion of the uterine crenel in pregnant animals, we explored whether this could exist due to a change in the capacity of the cervix to control microorganisms due to alteration in the expression and role of blueprint recognition receptors (TLRs), responsible for sensing microorganisms. The uterine cervix from non-significant and pregnant mice was analyzed for changes in TLR mRNA expression in the presence or absence of a systemic MHV68 infection. Systemic MHV68 viral infection, in the non-significant mice, either did not modify or increased the expression of specific TLRs (Fig. 3A). In dissimilarity, the cervix of meaning mice that had been exposed to MHV68 showed a substantial decrease in the expression of specific TLRs (Fig 3A–B).
MHV68 infection decreases TLR expression in the pregnant cervix
NT= no MHV68, MHV68= mice infected with virus. TLR mRNA expression was higher or did not change in the cervix of not significant MHV68 infected animals relative to not infected controls (A) but specific TLR mRNA was significantly decreased in the neck of MHV68-infected pregnant animals (B). Significance as denoted past confined is a p <.05. n=5
TLRs play a cardinal office in maintaining the control of microorganisms in the cervix by sensing microbial products and eliciting an innate immune response. To make up one's mind if these changes in TLRs gene expression resulted in functional differences in the capacity of the cervix to respond to bacterial infection, pregnant mice were either exposed to MHV68 or vehicle at pregnancy E8.five, followed past an intravaginal claiming of East. coli bacteria at E15.five of pregnancy. Since TLR ligation induces changes in cytokine/chemokine expression and AMP secretion, nosotros characterized the cervical cytokine/chemokine profile and AMP mRNA expression. We observed a robust pro-inflammatory cytokine response to leaner in the cervix of pregnant mice not exposed to MHV68 infections characterized past loftier tissue concentration of IL-1β, IL-6, KC, MCP-1, MIP-1α/β, IL12 and RANTES (Fig 4A–C). This cytokine/chemokine profile is stereotypic for a stiff pro-inflammatory anti-bacterial response. A dramatically different profile was observed in MHV68 infected pregnant animals. The presence of bacteria in the lower genital tract in MHV68 infected mice was not able to elicit a similar inflammatory response equally the one observed in mice, which received the same type of bacteria (Fig 4A–C). Indeed, the cervical protein concentration of IL-12, MIP-1α and β, RANTES and IL-6 of mice with MHV68 viral infection and bacteria were similar to those of the command group (non exposed to either bacteria or virus).
MHV68 infection reduces cytokine response to bacteria in the cervix
Cervical cytokines were measured using luminex technology; "NT" are cytokines from the cervix from animals that did not receive MHV68 or bacteria, "Bacteria" are cytokines from the cervix of animals with an intravaginal leaner injection, only no MHV68, and "MHV + Bacteria" are cytokines from the cervix of animals that received an intravaginal injection of bacteria while having an MHV68 infection. A number of cytokines and chemokines (A–C) were upregulated in the cervices of animals with artificial intravaginal bacterial infection, while this response was significantly reduced in animals with MHV68 infection. Beta defensin 1 (BD1), beta defensin three (BD3), beta defensin 4 (BD4) and beta defensin xiv (BD14) mRNA expression was also reduced in cervices from MHV68 infected animals (D). Significance is denoted by confined and is p <.05. n=five
In addition, AMP mRNA expression was lower in the pregnant neck of MHV68 infected mice than in that of significant animals not exposed to the virus (Fig 4D). These observations suggest that the decreased TLR gene expression in the cervix of MHV68 infected mice is associated with a lack of response to bacteria as demonstrated by the absence of pro-inflammatory cytokines and decreased expression of AMPs. These changes in the MHV68 infected pregnant mice may be functionally linked to the increased susceptibility to ascending bacterial infection.
Systemic assistants of MHV68 results in viral infection of the cervix of pregnant mice
The differences in the cervical response to viral and bacterial infections of meaning and non-pregnant mice could be attributed to variations in the systemic response to the virus or changes in cervical viral infection. To test this postulate, nosotros sought to determine if the virus was directly infecting the cervix. Meaning and non-pregnant mice received i.p. injections with MHV68 every bit described above; cervix and spleen samples were collected 7 days after injection and analyzed for MHV68 infection using qPCR for MHV68 ORF53. MHV68 viral infection was observed at similar concentrations in the spleen of pregnant and non-pregnant mice (Fig 5A), merely surprisingly, MHV68 viral infection was observed in the cervix of pregnant mice but was absent in the cervix of non-pregnant mice (Fig 5B). These results betoken pregnancy renders the uterine cervix susceptible to a systemic viral infection.
MHV68 infects the cervix of pregnant mice
Both pregnant and non-pregnant mice had similar systemic infections as determined by MHV68 ORF53 in the spleen (A), only pregnant mice also had loftier MHV68 titers in the cervix while not pregnant mice had no cervical infection (B). n=4, p<.001
Sexual practice hormones increment the susceptibility of the cervix to viral infection
Estrogen and progesterone are major factors associated with morphologic and functional changes of the cervix, during pregnancy(19). Since we plant that virus was only infecting the cervix of pregnant mice, we hypothesized high hormone concentrations during pregnancy induced modifications in the epithelium of the cervix that increase its susceptibility to viral infection. To examination this premise, we ovariectomized mice and they received hormone treatment [estradiol (500ng) and progesterone (500ug)] or placebo (vehicle) 21d post-surgery for 3d (Fig 6A) mimicking the hormonal status during pregnancy. Both handling groups so received injections of MHV68 i.p. and continued to get hormone therapy or vehicle every 2d for 7d (Fig 6A). Later, the cervix was collected and it was determined whether sex hormones made the cervix more susceptible to MHV68 infection. As suspected, MHV68 was detected in the cervix of animals receiving hormone therapy but not in ovariectomized mice receiving only vehicle (Fig 6B). These data suggest that hormonal changes associated with pregnancy induced modifications of the cervix leading to increased susceptibility to viral infection, and this could in plow bear upon the role of the uterine cervix in protecting against ascending bacterial infection.
Sex hormones play a role in MHV68 infection of neck tissue
Mice were overiectomized (OVX) and subsequently 3w, given either P4+E2 or vehicle for 3d; they were then injected with MHV68, and remained on either hormone treatments or vehicle for 7d (A). Seven days afterward infection, MHV68 was detected in the cervices of mice treated with hormones, but absent-minded in vehicle treated controls (B). n=4, p< .05
Integrins are increased in the cervix of pregnant mice and have a role in viral entry
Having determined that the high levels of sexual practice hormones found during pregnancy might increase the susceptibility of the cervix to viral infection, we hypothesized that this was due to increased expression of a protein or proteins on cervical cells that may act as a receptor for viral entry. Although the specific receptor for MHV68 entry is unknown, integrins are common entry receptors for related viruses (34, 35). To test the possibility that integrins are responsible for MHV68 infection of cervical cells we established an in vitro model using human ectocervical cells clone ECT1 that are permissive to MHV68 infection. Fibronectin is a high molecular weight glycoprotein nowadays in the extracellular matrix that binds to integrins (35), therefore, nosotros postulated that fibronectin would bind to integrins present in cervical cells and block viral entry. To test this premise, we incubated human cervical cells with fibronectin (500 ug/mL) followed past MHV68 infection. We observed a significant decrease in MHV68 infection in cells pre-treated with fibronectin compared to the non-fibronectin treated control, suggesting an integrin might exist involved in viral entry into cervical cells (Fig 7A). We then examined integrins in the neck of non-pregnant and pregnant mice to determine if their expression was correlated with MHV68 infectivity. Our data showed integrin blastoff 3 and beta 1 expression was positively correlated with MHV68 infection in the neck of infected significant (high expression) and not-meaning (low expression) mice (Fig 7B). This was not the case for integrin alpha 4, which was every bit expressed in non-pregnant and pregnant cervices (Fig 7B). Finally, to determine if integrin alpha 3, specifically, had a role in the susceptibility of MHV68 infection in the cervix, nosotros evaluated whether specific blocking antibodies for this integrin could prevent MHV68 viral infection, in vitro. Equally shown in figure 7C, we constitute that there was a pregnant decrease in the MHV68 titers in man cervical cells pre-treated with alpha 3 blocking antibody (Fig 7C) but not with the control IgG. Collectively, these data advise a possible mechanism whereby pregnancy can increase the susceptibility of the cervix to viral infection with MHV68.
Integrins play a function in MHV68 entry into cervical cells
Human being ectocervical cells (ECT1) were pretreated with fibronectin to cake integrin-ligand interactions and so infected with MHV68; 24h after infection, MHV68 was institute to exist partially blocked from cells treated with fibronectin (Fibronectin) compared to cells treated with MHV68 but no fibronectin (NT)(3 independent experiments) (A). Western blot analysis showed integrin alpha iii and beta one were upregulated in the pregnant cervix of infected mice (B) n=three. Antibodies blocking integrin alpha 3 (MHV68 + anti-integrin a3 ab) partially blocked MHV68 infection, while treatment with not specific IgG (MHV68 + IgG) did not cake MHV68 infection as compared to cells only treated with MHV68 (MHV68 only) (Representative of three independent experiments with a minimum of 3 animals per group) (C). Significance is denoted by bars and is p <.05.
Give-and-take
In the nowadays study we demonstrate, for the first time, that a viral infection of the neck, during pregnancy, reduces the capacity of the lower reproductive tract to foreclose bacterial infection of the meaning uterus. Furthermore, nosotros report that pregnancy increases the sensitivity of the cervix to viral infection leading to changes in the expression and office of TLRs and antimicrobial products. This sensitivity is partially caused by hormonal regulation of proteins in the neck that cause information technology to exist permissive to virus.
Approximately 30% of all neonatal death is directly acquired by preterm nascence and 50% of premature births are idiopathic (one, 36, 37). Since preterm birth represents a major health problem it is, therefore, of the greatest importance to determine its causes, which and then will allow us to develop novel ways for prevention and treatment. A strong trunk of evidence suggests that a majority of intrauterine bacterial infections during pregnancy outcome from bacteria ascending from the lower reproductive tract (2, six). The amniotic crenel is normally sterile and a major transition during life is the emergence from a sterile to a non-sterile environment at the fourth dimension of birth. Microbial invasion of the amniotic cavity can lead to preterm labor with intact membranes, preterm premature rupture of membranes, cervical insufficiency, a short neck, fetal sepsis, and preterm commitment. The presence of organisms in the amniotic crenel elicits an intense inflammatory response, which may evolve into a fetal inflammatory response syndrome. The latter predisposes preterm neonates to short- and long-term consequences such every bit neonatal sepsis, bronchopulmonary dysplasia, and cognitive palsy. Information technology has been estimated that one of every iii preterm neonates is built-in to a mother with intraamniotic infection, identified with either tillage or molecular microbiologic techniques (38).
Two major events demand to occur for bacteria to induce preterm labor: 1) bacteria need to breach the cervix and reach the decidua, amnion and potentially the fetus; 2) bacterial numbers must reach a threshold that volition trigger an inflammatory response that in turns induces preterm labor (39). A major question is how bacteria tin breach the cervical barrier and achieve the maternal-fetal interface. All women have microorganisms in the lower genital tract, nevertheless these microorganisms do not gain access to the amniotic crenel during normal pregnancy. What are the mechanisms responsible for preventing ascending intrauterine infection in about pregnant women? It is widely believed that the cervical mucus plug plays an of import role in host defense against microbial invasion of the amniotic cavity(xx, forty). Indeed, the cervical mucus plug has antimicrobial activity (41), contains antimicrobial peptides, as well equally immunoglobins and cellular components of the innate immune organization (macrophages, neutrophils, etc.) (42). Therefore, alterations of the composition or formation of the cervical plug may touch the protection against ascending leaner.
In this study nosotros start evaluated the regulation of leaner in the mouse FRT. We provide novel insights into the regulation of bacterial movement through the reproductive tract and reveal major differences depending on the reproductive phase. We observed, in our murine model, that bacteria delivered in the lower FRT is able to ascend to the uterine cavity confirming new findings in women, showing that the non meaning uterus has a normal flora (2, 43). On the other hand pregnant mice were able to forestall ascending bacteria from the lower FRT. These findings could suggest that bacteria in the upper FRT may not be a result of changes of the type of vaginal bacteria merely of the capacity of the cervix to regulate its ascension(44). These differences correlate with the biochemical and physical differences between the pregnant and not-pregnant cervix (20, 44).
A puzzling question has been why some significant women develop an ascending intraamniotic infection and others do non. In pregnancies complicated with bacterial infection, we propose that information technology is due to amending in the capacity of the cervix (lower FRT) to command leaner and non in the blazon of bacteria present in the vagina. In the nowadays study we demonstrate that under normal conditions, Ureaplasma urealyticum, the well-nigh common microorganism isolated in tissues from the maternal-fetal interface (6, 45) (31) is protected from the upper FRT past the cervix; however, if the cervix is infected with virus, the protection is decreased and U. urealyticum is able to accomplish the pregnant uterus. We advise that this reduced protection is due to the decrease in TLRs, antimicrobials and inflammatory cytokines in the neck infected with virus.
Pregnant women are more susceptible to the effects of viral infection than not-pregnant women. The mortality rate of pregnant women infected by influenza in the 1918 pandemic and in the nearly contempo H1N1 epidemic was significantly greater than that of non-significant women (46). This has been attributed to either an exaggerated inflammatory response (cytokine storm caused by the prime country of activation of the innate immune system during normal pregnancy) or secondary bacterial infections (47). The latter has been a field of study of involvement for many years and Dr. Luis Cruveilhier is cited to accept stated that "flu condemns, an additional infection executes" (48). Compelling evidence suggests that more ane microorganism causes many infectious diseases of humans and animals (49). Polymicrobial diseases are defined as pathologies acquired past the synergistic or sequential action of infectious agents from either the same or different kingdoms (49, l). Amongst the best known examples is the relationship between influenza and bacterial pneumonia. It is noteworthy that viral infections of the lower genital tract are relatively common (eastward.k. papilloma virus, herpes virus, HIV, etc.). Even so, there is a paucity of noesis well-nigh the effect of such localized infections on mucosal immunity of the lower genital tract during pregnancy (51). In this report we show for the first time that a viral infection could interfere in the normal anti-microbial office of the cervix during pregnancy.
In previous studies we used a murine gamma herpesvirus, MHV68 (29). This is a Dna virus of the same family as CMV and the HHVs, which have been found in the amnion, placenta and even the lower reproductive tract of significant women. These viruses all accept latency periods, produce immunosuppressive factors and many can exist reactivated by regulating TLRs function and expression. Naturally, MHV68 infects the nasopharyngeal tissue, leading to lytic infection and expansion in lung epithelial cells, followed past infection of B-cells, macrophages and dendritic cells, and viral latency (52). Interestingly, in our report, we constitute that information technology also infected the cervical cells of the pregnant mice. In humans, the most common viral infection of the cervix is human papillomavirus (HPV), and a handful of studies take shown that HPV infection of the placenta is associated with adverse pregnancy outcomes (53, 54). Even more recently, HPV infection of the cervix was related to placental abnormalities and preterm birth (55).
To understand why the cervix protection was compromised we commencement characterized the molecular response to viral infection. 1 of the main characteristics of the significant neck is the formation of the cervical plug, which is normally enriched with natural antimicrobial peptides such as alpha and beta defensins that tin can kill bacteria by damaging their outer barriers (xx) and recruit immune cells to the site of bacterial invasion. The epithelial cells further aid to protect against pathogens by the advisable expression of TLRs, secretion of cytokines and antimicrobial peptides (56, 57). Nosotros demonstrate that MHV68 infection of the cervix decreases TLR expression and consequently dampens the anti-microbial and inflammatory response to bacteria. This effect could exist part of the viral mechanism of evading host immune recognition. In contrast, TLR3, TLR9 and TLR2 are upregulated in the cervix of non-pregnant animals, potentially for heightened protection against viral infection. These results show that systemic infection regulates specific TLRs in mucosal epithelia quite differently, as compared to straight infection.
The pregnant state requires dramatic remodeling of the uterus. Sex steroid hormones and, in particular, estrogen and progesterone, take a powerful effect in remodeling the uterine cervix and the myometrium. Since only the pregnant cervix was infected by MHV68, this suggested that the changes of the neck are associated with the hormonal profile characteristic of pregnancy. This was confirmed with the observation that ovariectomized mice receiving estrogen and progesterone were more susceptible to viral infection of the cervix, suggesting that a systemic endocrine milieu can create conditions favoring viral invasion and multiplication. We were able to establish that integrin alpha 3 plays a role in the permissiveness of the cervix to MHV68 infection, although boosted factors may also be involved since the blocking studies did non completely diminish MHV68 infection.
Based on these findings nosotros propose the following model: commensal bacteria are located in the lower reproductive tract, and during salubrious pregnancy, the uterine cervix provides protection confronting leaner ascending into the upper reproductive tract (Fig 8A). If the protection provided by the uterine neck is jeopardized, bacteria can ascend from the lower tract, to the decidua and amnion, leading to inflammation and pregnancy complications such as preterm nascency (Fig 8B). In summary, these experiments are the first to describe a viral infection during pregnancy that alters the physiologic protection of the cervix against intrauterine infection. These studies also provide evidence that such changes are potentially mediated by contradistinct components of the innate immune response. Together our results propose that preterm labor is a polymicrobial disease, which requires a multifactorial approach for its prevention and treatment.
Model of polymicrobial illness during pregnancy
(A) Commensal bacteria are located in the lower reproductive tract, and during salubrious pregnancy, the uterine cervix provides protection against bacteria ascending into the upper reproductive tract. If the protection provided by the uterine cervix is jeopardized, bacteria can ascend from the lower tract, to the decidua and amnion, leading to inflammation and pregnancy complications such equally preterm nascence. We propose a model of polymicrobial disease during pregnancy: in this model, pregnancy and the associated sex hormones increment the susceptibility of the cervix to viral infection. Viral infection then results in a decrease in the protection confronting ascending bacteria. The subtract in protection can then atomic number 82 to intrauterine inflammation in response to bacteria and preterm nativity (B).
Acknowledgments
We acknowledge Dr. Michael Elowitz for the generous gift of the pZS2 plasmid used in this study and Melinda Wells for the model analogy.
Grant Back up This study is in part funded past grants from the National Institute of Health, NICDH P01HD054713 and 3N01 HD23342 and the Intramural Research Program of the Eunice Kennedy Shriver National Plant of Child Wellness and Human Evolution, National Institutes of Wellness, Section of Health and Homo Services
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Source: https://www.ncbi.nlm.nih.gov/pmc/articles/PMC4153356/
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