Scholarly article on topic 'Tissue-specific human beta-defensins (HBD)-1, HBD-2 and HBD-3 secretion profile from human amniochorionic membranes stimulated with Candida albicans in a two-compartment tissue culture system'

Tissue-specific human beta-defensins (HBD)-1, HBD-2 and HBD-3 secretion profile from human amniochorionic membranes stimulated with Candida albicans in a two-compartment tissue culture system Academic research paper on "Biological sciences"

Share paper
Academic journal
Reprod Biol Endocrinol
OECD Field of science

Academic research paper on topic "Tissue-specific human beta-defensins (HBD)-1, HBD-2 and HBD-3 secretion profile from human amniochorionic membranes stimulated with Candida albicans in a two-compartment tissue culture system"


Tissue-specific human beta-defensins (HBD)-1, HBD-2 and HBD-3 secretion profile from human amniochorionic membranes stimulated with Candida albicans in a two-compartment tissue culture system

Veronica Zaga-Clavellina1*, Martha Ruiz1, Pilar Flores-Espinosa1, Rodrigo Vega-Sanchez2, Arturo Flores-Pliego3, Guadalupe Estrada-Gutierrez4, Irma Sosa-Gonzalez4, Iyari Morales-Méndez4 and Mauricio Osorio-Caballero5

Background: During intrauterine infection, amniochorionic membranes represent a mechanical and immunological barrier against dissemination of infection. Human beta defensins (HBD)-1, HBD-2, and HBD-3 are key elements of innate immunity that represent the first line of defense against different pathogen microorganisms associated with preterm labor. The aim of this work was to characterize the individual contribution of the amnion (AMN) and choriodecidua (CHD) regions to the secretion of HBD-1, HBD-2 and HBD-3, after stimulation with Candida albicans. Methods: Full-thickness human amniochorionic membranes were obtained after delivery by elective cesarean section from women at 37-40 wk of gestation with no evidence of active labor. The membranes were cultured in a two-compartment experimental model in which the upper compartment is delimited by the amnion and the lower chamber by the choriodecidual membrane. One million of Candida albicans were added to either the AMN or the CHD face or to both and compartmentalized secretion profiles of HBD-1, HBD-2, and HBD-3 were quantified by ELISA. Tissue immunolocalization was performed to detect the presence of HBD-1, -2, -3 in tissue sections stimulated with Candida albicans.

Results: HBD-1 secretion level by the CHD compartment increased 2.6 times (27.30 [20.9-38.25] pg/micrograms protein) when the stimulus with Candida albicans was applied only on this side of the membrane and 2.4 times (26.55 [19.4-42.5] pg/micrograms protein) when applied to both compartments simultaneously. HBD-1 in the amniotic compartment remained without significant changes. HBD-2 secretion level increased significantly in the CHD when the stimulus was applied only to this region (2.49 [1.49-2.95] pg/micrograms protein) and simultaneously to both compartments (2.14 [1.67- 2.91] pg/micrograms protein). When the stimulus was done in the amniotic compartment HBD-2 remained without significant changes in both compartments. HBD-3 remained without significant changes in both compartments regardless of the stimulation modality. Localization of immune-reactive forms of HBD-1, HBD-2, and HBD-3 was carried out by immunohistochemistry confirming the cellular origin of these peptides.

Conclusion: Selective stimulation of amniochorionic membranes with Candida albicans resulted in tissue-specific secretion of HBD-1 and HBD-2, mainly in the CHD, which is the first region to become infected during an ascending infection.

* Correspondence:

department of Cell Biology, Instituto Nacionalde Perinatologia "Isidro

Espinosa de los Reyes", Mexico City, Mexico

Fulllist of author information is available at the end of the article


Bio Med Central

© 2012 Zaga-Clavellina et al.; licensee BioMed Central Ltd. This is an Open Access article distributed under the terms of the Creative Commons Attribution License (, which permits unrestricted use, distribution, and reproduction in any medium, provided the original work is properly cited.


During normal pregnancy, the human fetus must adapt to a potentially hostile environment in which both maternal and fetal tissues develop different and very complex adaptation strategies to avoid a potentially harmful response that can induce an alloimmune reaction between the mother and the fetus [1].

A growing body of clinical and experimental evidence supports the hypothesis that intrauterine infection during gestation is the principal causal factor in 25 to 40% of cases of preterm delivery; this condition jeopardizes the immunologic privilege of the fetus in the maternal-fetal interface, inducing an uncontrolled secretion of pro-inflammatory modulators that alter the immunologic/ endocrinologic equilibrium of the maternal-placental unit [2,3].

The amniotic cavity is a space delimited by amnio-chorionic membranes, that represent a physical as well as a very active immunologic barrier. These capacities are required to guarantee the effective response against any immunological challenge, including an effective prevention and eventual contention of microorganisms that reach the uterine cavity through an ascending pathway from the cervical-vaginal region [4].

Amniochorionic membranes are a complex bi-laminated tissue constituted by an amniotic epithelium whose cells are in contact with the amniotic fluid and by a chorion zone rich in chorion laeve trophoblasts attached to the maternal decidual lining of the uterine wall; all these cellular populations are embedded in an extracellular matrix rich in collagen types I, III, IV, V, and VI, as well as nidogen and proteoglycans [5,6].

The amniochorionic membranes are minimally vascu-larized; hence their immunologic capacities have been attributed -in part- to the innate immune system [7]. There is experimental evidence suggesting that the innate immune system plays a key role in the defense mechanisms against any immune and infectious challenge in the fetal-placental interface. Different studies support that amniochorionic membranes have intrinsic antibacterial properties [8-10].

Natural antimicrobial peptides (AMPs) are effector molecules of the innate immune system that have antibacterial (gram negative and gram positive bacteria), anti-viral, and anti-fungal actions; generally, they are constituted by 12-50 amino acid residues, and most of them are positively charged and have amphipathic properties [11,12]. These properties are important for their microbial killing mechanism: the cationic character of AMPs results in electrostatic attraction to the negatively-charged phospholipids of microbial membranes and their hydrophobicity aids in integrating them into the microbial cell membrane, leading to membrane disruption [11,13].

Defensins are an evolutionarily ancient class of AMPs present in animals, plants, and fungi [14]. Mammalian defensins can be subdivided into three main classes according to their structural differences: alpha-defensin, beta-defensin, and theta-defensin. Human beta defensins (HBD)-1,-2, -3, and -4 represent the main group of antimicrobials expressed at mucosal surfaces by epithelial cells [15].

Different natural AMPs play an active role during an infection process and the amniochorionic membranes are especially active in their production. There is clinical and experimental evidence indicating that: 1) primary amnion epithelial cells express messenger RNA for HBD-1 to 3, as well as secretory leukocyte protease inhibitor (SLPI) and elafin. Treatment with IL-|3 -a pro-inflammatory cytokine associated with labor in normal and pathological conditions- increases significantly HBD-2 [16]; 2). Stimulation of FL cells (ATCC CCL-62), a human amnion-derived line with LPS induces up-regulation of mRNA of HBD-3 [17]; 3) human amniotic epithelial cells (HAEC), isolated from human fetal membranes with chorioamnionitis, secrete significantly more HBD-3 after stimulation with LPS than cells isolated from normal pregnancy membranes [18]; 4) HBD-2 concentrations are increased in the amniotic fluid of women with microbial invasion of the amniotic cavity (MIAC) [19]; 5) the concentrations of immunoreactive a-defensins, human neutrophil peptides (HNP)-1-3, bactericidal/ permeability increasing protein (BPI), and calprotectin are significantly higher in patients with MIAC, preterm parturition, and preterm premature rupture of membranes (PPROM) [20]; 6) mRNA expression of alpha-defensin-1 and calgranulin B is significantly higher in fetal membranes of patients with preterm labor and histologic chorioamnionitis than in membranes of those without chorioamnionitis [21]; 7) elafin and HBD-3 increase in chorioamnionitis, and levels of HNP1-3 increase in plasma and amniotic fluid in women affected by microbial invasion of the uterus [22].

During pregnancy, HBD-1-3 plays a key role in the mechanisms that protect the maternal and fetal tissues and there is experimental evidence that they are expressed by the amnion's epithelium, decidual, placental, and chorion trophoblasts from term pregnancies [10]. Evidence from our laboratory indicates that chorioam-niotic membranes have tissue-specific capacities to synthesize and secrete HBDs. Using a two-compartment model of culture, we demonstrated that regardless of the primary site of stimulation with Streptococcus agalactiae, this bacterium induces secretion of HBD-2 and HBD-3 by both choriodecidual and amniotic regions; in contrast, HBD-1 remains without significant changes [23].

On the other hand, using the same experimental model, we demonstrated that Gardnerella vaginalis

induces secretion of HBD-1 mainly in the amniotic compartment, and HBD-2 and HBD-3 were secreted by the choriodecidual region [24]. Stimulation with Eshcerichia coli elicits a similar secretion HBD-2 profile in both choriodecidual and amniotic regions, however, HBD-3 was secreted mainly by the choriodecidual region but only if the stimulus was applied on the amniotic side [25].

Candida albicans is considered a microorganism associated with bacterial vaginosis, a condition that has been identified as a previous condition for the development of intrauterine and/or intra-amniotic infections [4,26]. Chorioamnionitis cases due to yeast colonization remain rare despite 10-20% rate of vaginal yeast colonize during pregnancy. A growing body of clinical evidence indicates, however, that C. albicans can be related with chorioamnionitis [27-29] and neonatal infections [26,30,31].

Epidemiological data indicate that 69-94% of neonates with a birth weight less than 1500 g die because of C. albicans-induced infections. Moreover, there are reports of fetal death during midgestation (18-21 weeks) associated to sepsis by C. albicans [31,32].

HBDs exhibit anti-fungal activity against Candidas spp, including C. albicans [33-35], therefore, the rationale for the present study was to test the individual contribution of the amnion and the choriodecidual regions to the secretion of HBD-1, -2, and -3 after stimulation with Candida albicans. Our findings suggest that HBD-1-3 may provide protection against penetration by microorganisms into the immune-privileged amniotic cavity.


Biological samples

The Internal Review Board of the Instituto Nacional de Perinatolgfa "Isidro Espinosa de los Reyes" (INPer IER) in Mexico City approved this study (#06151) and written informed consent was obtained from all participants.

Ten intact/whole term fetal membranes were collected from women who underwent elective cesarean section at term (37-39 weeks). All women were from an urban area of Mexico City, 23-34 years old, previously normoten-sive, with no history of diabetes mellitus, thyroid, liver, or chronic renal disease. They were cared for at the obstetrics out-patient service of the INPer IER. All women had uneventful pregnancies, with no evidence of active labor, cervical dilation or loss of the mucus plug. In addition, none had any clinical or microbiological signs of chorioamnionitis or of lower genital tract infection. Multi-fetal pregnancies were excluded from this study.

To confirm lack of infection, general microbiological analyses, including aerobic and anaerobic microorganisms, were conducted on the placenta and fetal membranes. Immediately after delivery, a sterile swab was rolled across randomly selected areas of the fetal membrane. The swabs were rolled onto Columbia agar

with 5% sheep blood, which was used as a primary isolation medium for fastidious and non-fastidious aerobic microorganisms.

Appropriate selective media were included for the detection of specific pathogens, e.g. MacConkey II agar (E. coli). Gardnerella selective agar with 5% human blood (G. vaginalis), potato dextrose agar (C. albicans), agar with 5% human blood (group B streptococci), and chocolate II agar (N. gonorrhoeae) were included.

A CDC anaerobic 5% sheep blood agar plate was streaked to isolate obligate and facultative anaerobes, as well as microaerophilic bacteria, using a Gas Pak EZ anaerobic system. All culture media were purchased from BD (Germany) and were incubated following the manufacturer's instruction. An additional swab was inoculated into Urea- Arginine LYO 2 broth (BioMerieux, Switzerland) to detect infection due to mycoplasma species.

Only membranes negative for aerobic and anaerobic microorganisms were used for this study.

Amniochorionic membranes explants culture

This model has been previoously validated and published by our group [36] and reproduced by others [37,38]. Briefly, all specimens were collected under aseptic conditions in the operating room and transported to the laboratory within 10 min of delivery in sterile Dulbecco's Modified Eagle Medium (DMEM) (Gibco BRL, Bethesda, MD) supplemented with 1X antibiotic-antimycotic solution (100 U/ml penicillin, 100 ^g/ml streptomycin) (Gibco) and rinsed in sterile saline solution (0.9% NaCl) to remove adherent blood clots.

Segments representing all zones of the membranes were manually cut into 14-18 mm diameter discs and held together with silicone rubber and placed on the upper chamber of a Transwell device, which were placed in the 12-well culture plates (Costar, New York, NY).

One milliliter of DMEM supplemented with 10% fetal bovine serum (FBS), 1 mM sodium pyruvate, and 1X antibiotic-antimycotic solution (100 U/ml penicillin, 100 ^g/ml streptomycin) (DMEM-FBS) (Gibco BRL) was added to each side of the chamber. The mounted explants were incubated in 5% CO2 at 37°C.

Explants stimulations

The first 24 hours in culture were used to stablize the membranes after manipulation. On the second day the membranes in both compartments are washed with saline solution (0.9% NaCl) to remove FBS. After washing, the explants were cultured with 1 ml of DMEM/com-partment suplemented with 0.2% of lactalbumin hydrol-ysate. Stimulation with the bacteria started immeditely upon addition of the culture medium.

Each experiment included the following set of chambers in triplicate: BASAL, control membranes in which 100 ^l of saline solution (vehicle) was added to both culture medium in both compartments of the chamber; CHORIODECIDUA (CHD), 1 x 106 CFU of Candida albicans was added only to the chorion compartment; AMNION (AMN), the yeast was added only to the amnion compartment; BOTH, the yeast stimulus was applied to both chorioamniotic and amniotic compartments simultaneously.

Co-incubation with C. albicans was done for 24 h, and the medium from both compartments of the chambers was collected and filtered (0.22 um); samples were aliquoted and stored at -70°C until assayed. All tissues were weighed and protein concentrations in all culture media were assessed with the Bradford method [39].

The inoculum size of 1 x 106 CFU has been pre-vioulsly standarized/published by our group to induce the secretion of a pro-inflammatory reaction, as well as the secretion of prostaglandin (PG)-E2 and matrix metalloprotease (MMP)-9 [40].

Measurement of HBD1, HBD2 and HBD3 secretion

Concentrations of HBD1, HBD2, and HBD3 were determined by enzyme-linked immunosorbent sandwich assays (ELISA) kits (Pepro Tech, Rock Hill, NJ). Standard curves used were as follows: HBD-1, 15 to 1000 pg/ ml with sensitivity of 4 pg/ml; HBD-2, 2 to 200 pg/ml with a detection limit of 1 pg/ml; and HBD-3, 10 to 2000 pg/ml with a sensitivity of 2 pg/ml.

Given that culture medium samples recovered from both compartments after stimulation did not contain fetal bovine serum and that these were filtered to remove any possible contamination with C. albicans and because HBD's are secreted to the medium, the final concentration of each HBD was expressed per microgram of the total protein concentration of each sample.


After stimulation with Candida albicans, the membranes were fixed, embedded in paraffin wax and 10-15 ^m sections were processed for immunohistochemical staining using the following polyclonal antibodies; rabbit anti-hHBD-1 and anti-hHBD-3, and a goat anti-hHBD-2 (Pepro Tech). The antibodies were used at a 10ug/ml dilution. The same membranes without stimulation were used as controls.

Binding of primary antibodies was detected using the avidin-biotinylated peroxidase technique and biotiny-lated horse anti-rabbit IgG and horse anti-goat IgG antibodies (Vector, Burlingame, CA). Tissue sections were counterstained with Mayer's hematoxylin and cover-slipped for evaluation by light microscopy.

Statistical analyses

Descriptive statistics (mean, standard deviation, standard error, median, and range) were obtained for each variable. Data distribution was tested for normality using Kolmogorov-Smirnoff and Shapiro-Wilk tests. When distribution was normal, Student's t test was used to analyze differences between treatments (i.e., control chorion vs stimulated chorion). Mann-Whitney's U test was used when data were not normally distributed. In every case, a P value < 0.05 was considered statistically significant. All statistical analyses were performed using SPSS 17 (IBM Corp., USA). Bars in the graphs represent median values and 25-75 interquartile range.


We evaluated HBD-1 secretion pattern in the culture medium after selective stimulation with C. albicans for 24 h. In comparison with basal secretion (11.57 [8.5116.29] pg/^g protein) in the choriodecidual compartment, stimulation of the choriodecidual side of the membrane induced, at least, a 2.5-fold increase (27.3 [20.9-38.25] pg/^g) of HBD-1 in this compartment. A similar pattern was induced when the stimulus was applied to both AMN and CHD simultaneously (26.55 [19.4-42.5] pg/^g of protein) Figure 1.

Stimulation at the amniotic side of the membrane did not induce significant changes of HBD-1 secretion profile (P = 0.107) in either AMN (10.36 [9.06-12.12] pg/^g of protein) or CHD (13.40 [10.82-20.07]) regions. In comparison with control conditions, CHD was the most active in the secretion of HBD-1 and the amniotic side did not respond in a significant way under any of the three infection modalities Figure 1.

Immunohistochemistry revealed an increase of im-munoreactive forms of HBD-1 after simultaneous stimulation of amnion and choriodecidua regions with C. albicans. The strongest HBD-1 signal was localized in the trophoblasts of the chorion. Distribution of HBD-1 signal was similar in all stimulation conditions Figure 2.

In comparison with basal levels, stimulation with C. albicans in the CHD region induced a significant increase of HBD-2 in both choriodecidual (2.49 [1.49-2.95] pg/^g of protein) and amniotic compartments (1.10 [0.85-1.20] pg/^g of protein). Yeast stimulation at the AMN side of the membrane did not induce any significant change (P = 0.25) in the pattern of HBD-2 secretion in either AMN or CHD Figure 3.

In comparison with basal levels in CHD (1.35 [0.991.92] pg/^g protein) and AMN (0.75 [ 0.53-0.96] pg/^g protein), simultaneous stimulation induced a significant increase of HBD-2 in chorionic and amniotic compartment (2.14 [1.67-2.91]) and (1.00-[0.9-1.13]) respectively Figure 3.

Figure 1 Compartamentalized in vitro secretion of HBD-1 after selective stimulation with Candida albicans. Antimicrobian peptide HBD-1 was measured in the medium from comparments delimited by the amnion (AMN) and the choriodecidua (CHD) under basalconditions and after the three different modalities of infection with 1 x 106 CFU of Candida albicans. Boxes represent median concentration of HBD-1 with 25-75 interquartile range; outlier values are represented by (•); (*P < 0.05, **P < 0.01, ***P < 0.001, n = 10). *Statistically different with respect to control value of choriodecidualcompartment.

Control tissues expressed immunoreactive forms of HBD-2 in the amniotic epithelium and trophoblast cells. Stimulation with C. albicans induced the increase of HBD-2 immunoreactive forms in both of these cells populations, especially within the choriodecidua region Figure 4.

ELISA assays indicated that HBD-3 concentration in the membranes stimulated with C. albicans were not significantly different from those found in basal conditions regardless of stimulation conditions Figure 5.

Immunolocalization of HBD-3 produced similar results Figure 6.


The immune innate system enables human amniochor-ionic membranes and other tissues of the fetal-maternal interface to recognize potentially infectious threats [41] and secrete AMP's that act as the first defense line to delimit and control an infectious process [10,15]. The key role of fetal membranes as an effective barrier against C.

Figure 2 Immunoreactivity of HBD-1 in human chorioamniotic membranes stimulated in both regions with C. albicans. The first panel shows a non-stimulated controlmembrane (a. 20X). Panelb shows HBD-1 immunoreactive forms in membranes stimulated simultaneously with C. albicans.

Chorion stimulus - + + - + +

Amnion stimulus - - - + + + +

Figure 3 Compartamentalized in vitro secretion of HBD-2 after selective stimulation with Candida albicans. Antimicrobian peptide HBD-2 was measured in the medium from comparments delimited by the amnion (AMN) and the choriodecidua (CHD) under basalconditions and after the three different modalities of infection with 1 x 106 CFU of Candida albicans. Boxes represent median concentration of HBD-2 with 25-75 interquartile range; outlier values are represented by (•); (*P < 0.05, **P < 0.01, ***P < 0.001, n =10). *Statistically different with respect to control values of the choriodecidualcompartment. #Statistically different with respect to controlvalues of the amniotic compartment.

albicans has been demonstrated in different animal experimental models [42,43].

Candida albicans has been identified as a microorganism isolated from the vagina, lower urinary tract, fetoplacental unit, and amniotic fluid during pregnancy and has been associated with an increased risk of premature rupture of membranes (PROM) and PPROM, which are associated with an increased risk of intra-amniotic infection; these are all conditions that negatively affect

perinatal morbidity and mortality of newborns [44]. Infants with a birth weight of less than 1250 g comprise the group with the highest risk of developing pulmonary candidiasis [45].

In a study addressed to know whether Candida species can penetrate intact fetal membranes under ex vivo conditions, it was possible to demonstrate that C. albi-cans was the only one that, once inoculated into the maternal side, penetrated and passed to the fetal side, and

Figure 4 Immunoreactivity of HBD-2 in human chorioamniotic membranes stimulated in both regions with C. albicans. The first panel shows a non-stimulated controlmembrane (a. 20X). Panelb shows HBD-2 immunoreactive forms in membranes stimulated simultaneously with C.aibicans.

Figure 5 Compartamentalized in vitro secretion of HBD-3 after selective stimulation with Candida albicans. Antimicrobian peptide HBD-3 was measured in the medium from comparments delimited by the amnion (AMN) and the choriodecidua (CHD) under basalconditions and after the three differente modalities of infection with 1 x 106 CFU of Candida albicans . Boxes represent median concentration of HBD-3with 25-75 interquartile range; outlier values are represented by (•); (*P < 0.05, **P < 0.01, ***P < 0.001, n = 10).

caused degeneration of the structure of the membrane epithelium [46].

In the present study, we addressed the question of whether the amniochorionic membranes are able to respond to Candida albicans infection with the production of HBD-1, HBD-2, HBD-3, peptides that directly combat bacterial proliferation and survival. The experimental model used in this study allowed us to reproduce the different contact points between Candida albicans,

ascending from the lower genital tract, and the uterine cavity; besides, we reproduced in vivo two compartments separated by a fully functional fetal membrane and analyzed the compartmentalized secretion in the compartment delimited by the amnion and that delimited by the choriodecidua [36].

The present work demonstrates that HBD-1 was the main defensin secreted by the membranes after stimulation with C. albicans. The ELISA and immunohistochemistry

a r I . [ ' « . • •. /, •. > 1 x . , V * b i i t * f - .•"< ' v ( ". ' j » j *

I J V ■ ' ■ ■ -si . " - -A * J t « * • -, ■ \ t • \ . 'i V.' ;, V 1 - \ 'vj ' ' ■ ■ . ' * * * * " * v . « ■V > 0 * * . t ' > M ' ■ /"A £ /.f

M i t ' i ° -, <> \ i1 t I

4 Rabbit IqG i >

Figure 6 Immunoreactivity of HBD-3 in human chorioamniotic membranes stimulated in both regions with C. albicans. The first panel shows a non-stimulated controlmembrane (a. 20X). Panelb shows HBD-3 membranes stimulated simultaneously with C.albicans.

results support the hypothesis that the choriodecidua is the region more active in the synthesis and secretion of this defensin.

These results are supported by previous evidence indicating that mRNA and protein of HBD-1 are present in the amnion, decidua, and chorion trophoblast layers of amniochorionic membranes, being the trophoblast region the main source of endogenous antimicrobial molecules during pregnancy [10].

Wiechula et al. [47] demonstrated that the mRNA of HBD-1 is increased in the lavage of female genital tract collected from women with candidiasis, which is in agreement with studies done with human normal vaginal epithelia co-cultured with C. albicans that induce a significant secretion of HBD-1 and HBD-2 [48].

The abundant secretion of HBD-1 in our model could be supported by a possible relationship between pregnancy tissues and the genitourinary tract, which expresses high levels of these defensins [14].

There are reports indicating that under pathological conditions, such as chorioamnionitis and/or PROM, which have been associated with uncontrolled production of harmful pro-inflammatory cytokines, the pattern of HBD-1 synthesis and secretion, as well as its immuno-localization profile, does not change [10]. However in a recent work in our laboratory, using the same experimental model of two independent compartments, we demonstrated that stimulation with G. vaginalis induces upregulation of HBD-1 [24].

In contrast, a growing body of evidence indicates that HBD-2 is up-regulated by inflammatory cytokines in cells derived from reproductive tissues, including fetal membranes [25] and in other organs, such as skin [49], human endometrial epithelial cells [50], oral epithelial cells [51,52], respiratory epithelia [53], and different colonic epithelial cell lines [54].

In the present work, we confirmed that HBD-2 is present at basal level in the membranes, which agrees with previous evidence reported by King et al. [10]. On the other hand, stimulation with C. albicans induced the increase of secreted levels and immuno-reactive forms of HBD-2 in both amniotic and choriodecidual compartments.

During pregnancy, HBD-2 is part of the immune machinery associated with the antimicrobial properties of the amniotic fluid; however, under pathological conditions such as MIAC, HBD-2 is up-regulated in the am-niotic fluid regardless of the fetal membrane status (intact membranes or PROM) [19]. These results concur with evidence of our lab indicating that the infection of fetal membranes with E. coli -a microorganism associated with chorioamnionitis- elicited high secretion of HBD-2 by both amnion and choriodecidua regions [25].

Additional evidence indicates that transcription of the HBD-2 gene is induced by IL-1|3 [54,55], a pro-inflammatory cytokine that is produced by the chorio-decidual region of human fetal membranes in response to a selective stimulation with C. albicans [40].

Additional experimental evidence indicate that HBD-2 elicits in vitro antifungal activity against Candida albicans, which is killed by a dose of 25 ^g/ml of HBD-2 that is lethal for 90% of strains tested (LD90) [54,56] and in an energy-dependent and salt-sensitive manner without causing membrane disruption [57].

HBD-3 is a 4-kDa antimicrobial peptide originally isolated from human psoriatic lesion scales [12] whose strong expression has been demonstrated in keratino-cytes and in tonsil tissue, whereas low HBD-3 expression was found in epithelia of the respiratory, gastrointestinal, and genitourinary tracts [58].

In the present study, we found that, independently from whether the yeast was added only to the amnion or to the choriodecidua or to both, stimulation with C. albicans did not induce any significant change in the HBD-3 secretion pattern, which was confirmed by immunohistochemistry.

It has been reported that HBD3 is up regulated by TNFa [59], however, previous evidence from our laboratory indicates that the stimulation of chorioamniotic membranes with C. albicans does not up-regulate the synthesis and secretion of TNFa [40].

Additionally, esophageal cell line OE21 stimulated with supernatants or directly co-cultured with C. albicans induces up-regulation of HBD-2 and HBD-3 expression, and the infection process involves divergent signaling events that differentially govern HBD-2 and HBD-3 [59]; these findings support our results indicating that the stimulation with C. albicans differentially up-regulates HBD-2 but not HBD-3, both defensins have been previously reported with strain-specific activity against Candida sp. including C. albicans [59,60].

Amniotic and choriodecidual regions are constituted by completely different cellular populations, which can explain -in part- the existence of tissue-specific HBD-1, HBD-2, and HBD-3 secretion patterns as part of the response to Candida albicans, this includes the basal protection of the three defensins and the up-regulation of HBD-1 and HBD-2 after stimulation with the yeast.

The present work and previous experimental evidence [23-25] support the concept that the human chorioam-niotic membranes have immune capacities that include innate immune factors, such as HBDs, that are secreted in a tissue specific pattern as part of a complex mechanism of defense/protection against different pathogen microorganisms associated to preterm labor complicated with chorioamnionitis. The action of these molecules may limit the spread of pathogens between maternal and

fetal compartments preventing the infection of the am-niotic cavity.

Innate immune capacities in pregnancy tissues are key in the recognition, delimitation, and eventual destruction of pathogens that can damage the immunologic equilibrium at the maternal-placental interface. Differential capacities to recognize the pathogen are directly associated with receptors of the innate immune system, Toll like receptors (TLRs) are a family of pattern recognition receptors that respond to the presence of pathogen-derived products and are responsible in part for the control of antimicrobial expression [61,62].

There is evidence supporting the active role of the innate immune system, TLR-4 and TLR-2 are two key receptors in the recognition of linear structure of O-linked mannosyl residues [63] and |3-(1,3)-mannosides, which are present in the acid-stable and acid-labile component of mannoproteins and phospholipomannans (PLM) [64] on the Candida albicans cell wall, respectively. Additionally fungal DNA is poorly methylated in contrast to mammalian DNA, and experimental evidence indicates that TLR-9 is involved in the recognition of C. albicans [62,65].

At the maternal-placental interface, TLRs play a key role as sentinels to detect different pathogens, these receptors are expressed not only in the immune cells but also in non-immune cells, including amniotic epithelium, villous and extra-villous trophoblasts, and decidual cells, and their expression pattern can vary according to the stage of pregnancy [61,62].

The expression and activity of TLR-2 and TLR-4 have been associated with spontaneous labor at term, as well as with preterm delivery with histological chorioamnio-nitis, indicating that these receptors play a key role in the innate immune mechanisms required to respond effectively against an immunologic-infectious process [61].


Our results demonstrate that amniochorionic membranes respond differentially to Candida albicans infection. Amnion and choriodecidua secrete HBD-1 and HBD-2 as part of the innate immune defenses of this tissue.

The choriodecidua is the most responsive region to the infection, as it is the first tissue to be colonized by the microbial pathogen during an ascending intrauterine infection and it is the main barrier to progression of the infection into the amniotic cavity and eventually the fetus.

Tissue-specific capacities of these membranes to secret HBD-1 and HBD-2 represent the first line of defense in amniochorionic membranes and represent part of a very complex mechanism of antimicrobial protection that

ensures an initial protection at times when infection may jeopardize the continuity of pregnancy.


AMN: Amnion; AMP: Naturalantimicrobialpeptides; BPI: Bactericidal permeability increasing protein; CHD: Choriodecidua; CFU: Colony forming unit; DMEM: Dulbecco modified eagle medium; ELISA: Enzyme-linked immunosorbent assay; FBS: Fetalbovine serum; HBD: Human beta defensins; HEC: Human amniotic epithelialcells; HNP: Human neutrophilpeptide; LPS: Lipopolysacharide; MIAC: Microbialinvasion of the amniotic cavity; PROM: Premature rupture of membranes; SLPI: Secretory leukocyte protease inhibitor; TLR: Tolllike receptors.

Competing interests

The authors declare that they have no competing interests. Authors' contributions

VZC, MR, PFE, MOC, and AFP collected the samples, culture membranes, performed stimulation with the bacterium and ELISA assays. GEG and RVS performed the statisticalanalyses. ISG and IMM performed the microbiologicalcontrol. VZC and MR participated in the design of the study, data collection, and analysis, as wellas manuscript preparation. Allauthors have read and approved the finalmanuscript.


These studies were supported by Instituto Nacionalde Perinatologia "Isidro Espinosa de los Reyes", project # 06151 to VZC. We thank Ingrid Mascherfor editorial assistance and Dr. Daudi Langat and David Wheaton for language corrections.

Author details

department of Cell Biology, Instituto Nacionalde Perinatologia "Isidro Espinosa de los Reyes", Mexico City, Mexico. 2Department of Nutrition Research, Instituto Nacionalde Perinatologia "Isidro Espinosa de los Reyes", Mexico City, Mexico. 3Department of Biochemistry and Molecular Biology, Instituto Nacionalde Perinatologia "Isidro Espinosa de los Reyes", Mexico City, Mexico. 4Department of Infectology, Instituto Nacionalde Perinatologia "Isidro Espinosa de los Reyes", Mexico City, Mexico. 5Department of Family Planning, Department of Gynecology and Obstetrics, Instituto Nacionalde Perinatologia "Isidro Espinosa de los Reyes", Mexico City, Mexico.

Received: 8 June 2012 Accepted: 27 August 2012 Published: 3 September 2012


1. Levy O: Innate immunity of the newborn: basic mechanisms and clinical correlates. Nat Rev Immunol 2007, 7:379-390.

2. Yoon BH, Romero R, Moon JB, Shim SS, Kim M, Kim G, Jun JK: Clinical significance of intra-amniotic inflammation in patients with preterm labor and intact membranes. Am J Obstet Gynecol 2001, 185:1130-1136.

3. Asrat T: Intra-amniotic infection in patients with preterm prelabor rupture of membranes. Pathophysiology, Detection, and Management. Clinic Perinatal 2001, 28:735-751.

4. Romero R, Mazor M: Infection and preterm labor. Clin Obstet Gynecol 1988, 31:553-584.

5. Parry S, Strauus JF: Premature rupture of the fetal membranes. N Engl J

Med 1998, 338:663-668.

6. Malak TM, Ockleford CD, Bell SC, Dalgleish R, Bright N, Macvicar J: Confocal immunofluorescence localization of collagen types I, III, IV, V and VI and their ultrastructural organization in term human fetal membranes.

Placenta 1993,14:385-406.

7. Klein LL, Gibbs RS: Infection and preterm birth. Obstet Gynecol Clin North Am 2005, 32:397-410.

8. Talmi YP, Sigler L, Inge E, Finkelstein Y, Zohar Y: Antibacterial properties of human amniotic membranes. Placenta 199,12:285-288.

9. Kjaergaard N, Hein M, Hyttel L, Helmig RB, Sch0nheyder HC, Uldbjerg N, Madsen H: Antibacterial properties of human amnion and chorion

in vitro. Eur J Obstet Gynecol Reprod Biol 2001, 94:224-229.

10. King AE, Paltoo A, Kelly RW, Sallenave JM, Bocking AD, Challis JR: Expression of natural antimicrobials by human placenta and fetal membranes. Placenta 2007, 28:161-169.

11. Hancock RE, Diamond G: The role of eationie antimicrobial peptides in innate host defences. Trends Microbiol 2000, 8:402-410.

12. De Smet K, Contreras R: Human antimicrobial peptides: defensins, cathelicidins and histatins. Biotechnol Lett 2005, 27:1337-1347.

13. Yeaman MR, Yount NY: Mechanisms of antimicrobial peptide action and resistance. Pharmacol Rev 2003, 55:27-55.

14. Ganz T, Selsted ME, Szklarek D, Harwig SS, Daher K, Bainton DF, Lehrer RI: Defensins. Natural peptide antibiotics of human neutrophils. J Clin Invest 1985, 76:1427-1435.

15. Schneider JJ, Unholzer A, Schaller M, Schäfer-Korting M, Korting HC: Human defensins. J Mol Med (Berl) 2005, 83:587-595.

16. Stock SJ, Kelly RW, Riley SC, Calder AA: Natural antimicrobial production by the amnion. Am J Obstet Gynecol 2007, 196:255.e1-255.e6.

17. Buhimschi IA, Jabr M, Buhimschi CS, Petkova AP, Weiner CP, Saed GM: The novel antimicrobial peptide beta3-defensin is produced by the amnion: a possible role of the fetal membranes in innate immunity of the amniotic cavity. Am J Obstet Gynecol 2004, 191:1678-1687.

18. Szukiewicz D, Szewczyk G, Pyzlak M, Klimkiewicz J, Maslinska D: Increased production of beta-defensin 3 (hBD-3) by human amniotic epithelial cells (HAEC) after activation of toll-like receptor 4 in chorioamnionitis. Inflamm Res 2008, 57(Suppl 1):S67-S68.

19. Soto E, Espinoza J, Nien JK, Kusanovic JP, Erez O, Richani K, Santolaya-Forgas J, Romero R: Human beta-defensin-2: a natural antimicrobial peptide present in amniotic fluid participates in the host response to microbial invasion of the amniotic cavity. J Matern Fetal Neonatal Med 2007, 20:15-22.

20. Espinoza J, Chaiworapongsa T, Romero R, Edwin S, Rathnasabapathy C, Gomez R, Bujold E, Camacho N, Kim YM, Hassan S, Blackwell S, Whitty J, Berman S, Redman M, Yoon BH, Sorokin Y: Antimicrobial peptides in amniotic fluid: defensins, calprotectin and bacterial/permeability-increasing protein in patients with microbial invasion of the amniotic cavity, intra-amniotic inflammation, preterm labor and premature rupture of membranes. J Matern Fetal Neonatal Med 2003,13:2-21.

21. Erez O, Romero R, Tarca AL, Chaiworapongsa T, Kim YM, Than NG, Vaisbuch E, Draghici S, Tromp G: Differential expression pattern of genes encoding for anti-microbial peptides in the fetal membranes of patients with spontaneous preterm labor and intact membranes and those with preterm prelabor rupture of the membranes. J Matern Fetal Neonatal Med 2009, 22:1103-1115.

22. King AE, Kelly RW, Sallenave JM, Bocking AD, Challis JR: Innate immune defences in the human uterus during pregnancy. Placenta 2007, 28:1099-1106.

23. Zaga-Clavellina V, Garcia-Lopez G, Flores-Espinosa P: Evidence of in vitro differential secretion of human beta-defensins-1, -2, and -3 after selective exposure to Streptococcus agalactiae in human fetal membranes. J Matern Fetal Neonatal Med 2012,4:258-263.

24. Zaga-Clavellina V, Martha RV, Flores-Espinosa P: In vitro secretion profile of pro-inflammatory cytokines IL-1 ß, TNF-a, IL-6, and of human beta-defensins (HBD)-1, HBD-2, and HBD-3 from human chorioamniotic membranes after selective stimulation with Gardnerella vaginalis. Am J Reprod Immunol 2012, 67:34-43.

25. Garcia-Lopez G, Flores-Espinosa P, Zaga-Clavellina V: Tissue-specific human beta-defensins (HBD)1, HBD2, and HBD3 secretion from human extra-placental membranes stimulated with Escherichia coli. Reprod Biol Endocrinol 2010, 8:146.

26. Donders GG, Moerman P, Caudron J, Van Assche FA: Intra-uterine Candida infection: a report of four infected fetusses from two mothers. Eur J Obstet Gynecol Reprod Biol 1991, 38:233-238.

27. Romero R, Reece EA, Duff GW, Coultrip L, Hobbins JC: Prenatal diagnosis of Candida albicans chorioamnionitis. Am J Perinatol 1985, 2:121-122.

28. Bruner JP, Elliott JP, Kilbride HW, Garite TJ, Knox GE: Candida chorioamnionitis diagnosed by amniocentesis with subsequent fetal infection. Am J Perinatol 1986, 3:213-218.

29. Berry DL, Olson GL, Wen TS, Belfort MA, Moise KJ Jr: Candida chorioamnionitis: a report of two cases. J Matern Fetal Med 1997, 6:151-154.

30. Baley JE: Neonatal candidiasis: the current challenge. Clin Perinatol 1991, 18:263-280.

31. Ng PC, Siu YK, Lewindon PJ, Wong W, Cheung KL, Dawkins R: Congenital Candida pneumonia in a preterm infant. J Paediatr Child Health 1994, 30:552-554.

Engelhart CM, van de Vijver NM, Nienhuis SJ, Hasaart TH: Fetal Candida sepsis at midgestation: a case report. Eur J Obstet Gynecol Reprod Biol 1998, 77:107-109.

Krishnakumari V, Rangaraj N, Nagaraj R: Antifungal activities of human

beta-defensins HBD-1 to HBD-3 and their C-terminal analogs Phd1 to

Phd3. Antimicrob Agents Chemother 2009, 53:256-260.

Feng Z, Jiang B, Chandra J, Ghannoum M, Nelson S, Weinberg A: Human

beta-defensins: differential activity against candidal species and

regulation by Candida albicans. J Dent Res 2005, 8:445-450.

Lupetti A, Danesi R, Wout JW V't, Van Dissel JT, Senesi S, Nibbering PH:

Antimicrobial peptides: therapeutic potential for the treatment of

Candida infections. Expert Opin Investig Drugs 2002, 11:309-318.

Zaga V, Estrada-Gutierrez G, Beltran-Montoya J, Maida-Claros R,

Lopez-Vancell R, Vadillo-Ortega F: Secretions of interleukin-1 beta and

tumor necrosis factor alpha by whole fetal membranes depend on initial

interactions of amnion or choriodecidua with lipopolysaccharides or

group B streptococci. Biol Reprod 2004, 71:1296-1302.

Thiex NW, Chames MC, Loch-Caruso RK: Tissue-specific cytokine release

from human extra-placental membranes stimulated by

lipopolysaccharide in a two-compartment tissue culture system. Reprod

Biol Endocrinol 2009, 7:117.

Miller MF, Loch-Caruso R: Comparison of LPS-stimulated release of cytokines in punch versus transwell tissue culture systems of human gestational membranes. Reprod Biol Endocrinol 2010, 8:121. Bradford MM: A rapid and sensitive method for the quantitation of microgram quantities of protein utilizing the principle of protein-dye binding. Anal Biochem 1976, 72:248-254.

Zaga-Clavellina V, Lopez GG, Estrada-Gutierrez G, Martinez-Flores A, Maida-Claros R, Beltran-Montoya J, Vadillo-Ortega F: Incubation of human chorioamniotic membranes with Candida albicans induces differential synthesis and secretion of interleukin-1beta, interleukin-6, prostaglandin E, and 92 kDa type IV collagenase. Mycoses 2006, 49:6-13. Abrahams VM: Pattern recognition at the maternal-fetal interface. Immunol Invest 2008, 37:427-447.

Gow NA, Knox Y, Munro CA, Thompson WD: Infection of chick chorioallantoic membrane (CAM) as a model for invasive hyphal growth and pathogenesis of Candida albicans. Med Mycol 2003, 41:331-338. Jacobsen ID, Grosse K, Berndt A, Hube B: Pathogenesis of Candida albicans infections in the alternative chorio-allantoic membrane chicken embryo model resembles systemic murine infections. PLoS One 2011, 6:e19741. Velemfnsky M, Tosner J: Relationship of vaginal microflora to PROM, pPROM and the risk of early-onset neonatal sepsis. Neuro Endocrinol Lett 2008, 29:205-221.

Frezza S, Maggio L, De Carolis MP, Gallini F, Puopolo M, Polimeni V, Costa S, Vento G, Tortorolo G: Risk factors for pulmonary candidiasis in preterm infants with a birth weight of less than 1250 g. Eur J Pediatr 2005, 164:88-92.

Gurgan T, Diker KS, Haziroglu R, Urman B, Akan M: In vitro infection of human fetal membranes with Candida species. Gynecol Obstet Invest 1994, 37:164-167.

Wiechuta B, Cholewa K, Ekiel A, Romanik M, Dolezych H, Martirosian G: HBD-1 and hBD-2 are expressed in cervico-vaginal lavage in female genital tract due to microbial infections. Ginekol Pol 2010, 81:268-271. Liu Z, Chen L: Congenital anti-candida of human vaginal epithelial cells.

Beijing Da Xue Xue Bao. 2008, 40:174-177.

S0rensen OE, Thapa DR, Rosenthal A, Liu L, Roberts AA, Ganz T: Differential regulation of beta-defensin expression in human skin by microbial stimuli. J Immunol 2005, 174:4870-4879.

King AE, Fleming DC, Critchley HO, Kelly RW: Regulation of natural antibiotic expression by inflammatory mediators and mimics of infection in human endometrial epithelial cells. Mol Hum Reprod 2002, 8:341-349. Krisanaprakornkit S, Kimball JR, Weinberg A, Darveau RP, Bainbridge BW, Dale BA: Inducible expression of human beta-defensin 2 by Fusobacterium nucleatum in oral epithelial cells: multiple signaling pathways and role of commensal bacteria in innate immunity and the epithelial barrier. Infect Immun 2000, 68:2907-2915. Mathews M, Jia HP, Guthmiller JM, Losh G, Graham S, Johnson GK, Tack BF, McCray PB Jr: Production of beta-defensin antimicrobial peptides by the oral mucosa and salivary glands. Infect Immun 1999, 67:2740-2745. Harder J, Meyer-Hoffert U, Teran LM, Schwichtenberg L, Bartels J, Maune S, Schroder JM: Mucoid Pseudomonas aeruginosa, TNF-alpha, and IL-1beta,

but not IL-6, induce human beta-defensin-2 in respiratory epithelia. Am J

Respir Cell Mol Biol 2000, 22:714-721.

54. O'Neil DA, Porter EM, Elewaut D, Anderson GM, Eckmann L, Ganz T, Kagnoff MF: Expression and regulation of the human beta-defensins hBD-1 and hBD-2 in intestinal epithelium. J Immunol 1999, 163:6718-6724.

55. Schröder JM, Harder J: Human beta-defensin-2. Int J Biochem Cell Biol 1999, 31:645-651.

56. Hiemstra PS: Epithelial antimicrobial peptides and proteins: their role in host defence and inflammation. Paediatr Respir Rev 2001, 2:306-310.

57. Vylkova S, Nayyar N, Li W, Edgerton M: Human beta-defensins kill Candida albicans in an energy-dependent and salt-sensitive manner without causing membrane disruption. Antimicrob Agents Chemother 2007, 51:154-161.

58. Harder J, Bartels J, Christophers E, Schroder JM: Isolation and characterization of human beta -defensin-3, a novel human inducible peptide antibiotic. J Biol Chem 2001, 276:5707-5713.

59. Steubesand N, Kiehne K, Brunke G, Pahl R, Reiss K, Herzig KH, Schubert S, Schreiber S, Fölsch UR, Rosenstiel P, Arlt A: The expression of the beta-defensins hBD-2 and hBD-3 is differentially regulated by NF-kappaB and MAPK/AP-1 pathways in an in vitro model of Candida esophagitis. BMC Immunol 2009, 10:36.

60. Joly S, Maze C, McCray PB Jr, Guthmiller JM: Human beta-defensins 2 and 3 demonstrate strain-selective activity against oral microorganisms. J Clin Microbiol 2004, 42:1024-1029.

61. Kim YM, Romero R, Chaiworapongsa T, Kim GJ, Kim MR, Kuivaniemi H, Tromp G, Espinoza J, Bujold E, Abrahams VM, Mor G: Toll-like receptor-2 and -4 in the chorioamniotic membranes in spontaneous labor at term and in preterm parturition that are associated with chorioamnionitis. Am J Obstet Gynecol 2004, 191:1346-1355.

62. Patni S, Flynn P, Wynen LP, Seager AL, Morgan G, White JO, Thornton CA: An introduction to Toll-like receptors and their possible role in the initiation of labour. BJOG 2007, 114:1326-1334.

63. Netea MG, Gow NA, Munro CA, Bates S, Collins C, Ferwerda G, Hobson RP, Bertram G, Hughes HB, Jansen T, Jacobs L, Buurman ET, Gijzen K, Williams DL, Torensma R, McKinnon A, MacCallum DM, Odds FC, Van der Meer JW, Brown AJ, Kullberg BJ: Immune sensing of Candida albicans requires cooperative recognition of mannans and glucans by lectin and Toll-like receptors. J Clin Invest 2006, 116:1642-1650.

64. Jouault T, El Abed-El Behi M, Martínez-Esparza M, Breuilh L, Trinel PA, Chamaillard M, Trottein F, Poulain D: Specific recognition of Candida albicans by macrophages requires galectin-3 to discriminate Saccharomyces cerevisiae and needs association with TLR2 for signaling. J Immunol 2006, 177:4679-4687.

65. Bellocchio S, Montagnoli C, Bozza S, Gaziano R, Rossi G, Mambula SS, Vecchi A, Mantovani A, Levitz SM, Romani L: The contribution of the Toll-like/IL-1 receptor superfamily to innate and adaptive immunity to fungal pathogens in vivo. J Immunol 2004, 172:3059-3069.


Cite this article as: Zaga-Clavellina et al.: Tissue-specific human beta-defensins (HBD)-1, HBD-2 and HBD-3 secretion profile from human amniochorionic membranes stimulated with candida albicans in a two-compartment tissue culture system. Reproductive Biology and Endocrinology 2012 10:70.

Submit your next manuscript to BioMed Central and take full advantage of:

• Convenient online submission

• Thorough peer review

• No space constraints or color figure charges

• Immediate publication on acceptance

• Inclusion in PubMed, CAS, Scopus and Google Scholar

• Research which is freely available for redistribution

Submit your manuscript at Tpntral >_ciiuai