Elevated Birth Rates in CD62L (L-Selectin)-Deficient BALB/c Mice: Potential Involvement of NK Cells ()
1. Introduction
Uterine implantation of the human embryo begins with attachment of the blastocyst to the trophoblast. Because this process occurs under conditions of shear stress it parallels leukocyte transmigration, suggesting that the molecular basis of these processes might be analogous. Numerous investigators (and our previous studies) have confirmed a key role for leukocyte (L)-selectin (CD62L) in the inflammatory processes. CD62L plays a key first step in initiating leukocyte migration from specialized blood vessels (high endothelial venules) into the lymph node parenchyma following L-selectin binding to carbohydrate rich ligands. Outside the lymph node this interaction facilitates chemokine-driven leukocyte transmigration into inflamed tissues [1] - [3] . The same L-selectin adhesion system (L-selectin and its carbohydrate rich ligands) has been implicated in initial embryo-maternal interactions [4] - [6] and L-selectin/ligand binding has been suggested to be critical to uterine trophoblast cell development [7] .
Although the mouse trophectoderm expresses L-selectin, its carbohydrate rich ligands (especially sulfated carbohydrates) are missing from the murine luminar and glandular epithelium at this developmental stage suggesting that other integrins and/or adhesion molecules may play a role in mediating this interaction [7] - [10] .
Recently, we found that CD62L-deficient BALB/c mice delivered unexpectedly larger litters compared to wild type (WT) BALB/c mice. This observation led us to investigate the role of L-selectin in fetal survival and implantation. Due to the lack of adhesion molecules like L-selectin critical to leukocyte migration and extravasation, the goal of the current study was to characterize the immune cells present at the fetal-maternal interface and to define potential mechanism(s) associated with increased birth rates in CD62L-deficient mice by comparing uterine tissue samples harvested during the early stages of pregnancy.
2. Methods
2.1. Reagents
All chemicals unless otherwise specified were purchased from Sigma Chemical Co. (St. Louis, MO) or Fischer Scientific (Chicago, IL). Phosphate-buffered saline (PBS; pH 7.4) was used for washing and short-term storage of cells until use. Cell-surface labeling with monoclonal antibodies (mAb) was carried out in flow cytometry wash buffer (PBS containing 0.1% NaN3 and 0.1% bovine serum albumin).
2.2. Mice and Tissue Collection
This study was approved by the Institutional Animal Care and Use Committee (IACUC) at Rush University Medical Center. BALB/c mice were purchased from the Charles River Laboratories (Wilmington, MA). CD62L-deficient mice were purchased from The Jackson Laboratories and backcrossed into the BALB/c background as described earlier and housed under pathogen-free conditions [2] . A total of 43, 8 - 10-week-old WT BALB/c female (n = 18) mice and L-selectin-deficient female mice (n = 25) were selected based on estrus-based vaginal smear checks conducted daily and then paired with age-matched CD62L-deficient or control WT BALB/c males. To standardize pregnancy age, males were kept only for 1 night in the breeding cages. Detection of a vaginal plug was defined as gestation day (GD) 0. Pregnant mice were sacrificed using CO2 asphyxiation on GD 9.5 and uterine tissues harvested immediately, perfused with PBS, dissected, and digested with collagenase D (2 mg/ml in PBS).
2.3. Histological Procedures
Formalin-fixed GD 9.5 implantation sites were embedded in paraffin and 7 μm transverse sections were stained with hematoxylin and eosin (H & E). The H&E-stained sections were examined under bright-field light microscopy.
For immunofluorescence staining, tissue sections were incubated in 10% normal goat serum in PBS for 60 min and then incubated with either PE- or FITC-conjugated individual primary antibodies Abs (BD biosciences, San Jose, CA, USA) for 60 min. The following Abs were used: anti-GR-1 (for neutrophil detection), anti- MECA-32 or anti-E-selectin (for mouse endothelium detection), anti-CD3 (for T cell detection), and rat anti- mouse B220 (for B cell detection). For uterine NK cells, Dolichos biflorus agglutinin (DBA) lectin staining was used. Samples were washed with PBS for 30 min and analyzed under epifluorescent microscopy (Nikon, Microphot FMX).
2.4. Flow Cytometric Analysis of the Fetal-Maternal Interface
Fluorochrome-labeled rat anti-mouse antibodies specific for NK cells (anti-CD3-LFA-1+ Thy 1.2+), granulocytes (anti-GR1, anti-CD11b, anti-F4/80), B cells (rat anti-mouse B220), and T cells (anti-CD3) were purchased from BD Biosciences (San Jose, CA). We used multicolor labeling for the simultaneous detection of cell surface molecules on cells harvested from mouse uterine tissues at GD 9.5. Samples obtained from uterine segments (conceptus) containing the developing embryo were harvested, homogenized, and then measured using a FACS Canto II flow cytometer and data analyzed using FACS DIVA software (BD Flow Cytometry Systems, San Jose, CA). Specific cell populations were expressed as the percent of total cells unless otherwise specified. Fluorescence histogram plots were used to compare mean fluorescence intensities (MFIs) of different samples and to calculate the proportion of cells staining positive.
2.5. Statistical Analysis
Statistical analyses were performed using IBM SPSS Statistic 20 (IBM Corporation) at the Rush University Medical Center, Chicago, USA. The comparisons were made between the four breeding groups and the mean litter sizes according to the Mann-Whitney U test. To evaluate differences between the mean number of lymphocytes localized at the uterine segments in both, wild type, and CD62L−/− mice Kolmogorov-Smirnov non- parametric test was applied. Mean data are reported ± standard error of the mean (SEM). Statistical significance was set at (*) p < 0.05, or (**) p < 0.1.
3. Results
3.1. Litter Numbers
To determine whether the L-selectin deficiency in either males or females was responsible for the observed increase in litter sizes and to determine the average number of viable pups, we performed a comparative breeding analysis using 10-week-old nulliparous BALB/c mice. The following breeding pair combinations were established: (1) CD62L-deficient females and CD62L-deficient males (n = 14 breeding pairs), (2) CD62L-deficient females and WT males (n = 11 breeding pairs), (3) WT females and CD62L-deficient males (n = 8 breeding pairs), and (4) WT females and WT males (n = 10 breeding pairs). CD62L-deficient male and CD62L-deficient female crossings produced 118 pups with an average number of 8.43 ± 0.55 SEM pups/litter (Figure 1). CD62L-deficient females crossed with WT males delivered 92 pups with an average number of 8.36 ± 0.77 SEM pups/litter (Figure 1). WT females crossed with CD62L-deficient males had 80 pups with an average number of 6.66 ± 0.8 SEM pups/litter (Figure 1). WT breeding pairs produced 49 pups with an average number of 6.12 ± 0.3 pups/litter SEM (Figure 1). We observed a statistically significant difference between the size of the litter obtained from CD62L-deficient (male × female) breeding pairs compared to WT male x WT female breading pairs (p < 0.01) and WT female × CD62L-deficient male breading pairs (p < 0.05). These data clearly demonstrated that the significantly increased litter size observed was impacted by CD62L-deficiency in females (Figure 1). Pups obtained from all breading pairs were healthy and viable and no significant differences between the weights or lengths of pups derived from any breading pairs were observed even at 3 weeks of age (Table 1). Pups obtained from all breeding pairs developed normally and were fertile 8 weeks after birth (Table 1).
Figure 1. Average litter numbers. Columns demonstrate the mean litter numbers of viable pups, derived from four combinations of breeding pairs. Error bars represent the standard error of mean. *p < 0.05, **p < 0.
Table 1. Neonatal outcome, survival rates, weights and lengths of mice.
3.2. Flow Cytometric Assessment of Leukocytes Surrounding the Developing Embryos
A profile of the type of immune cells present in uterine segments containing a developing embryo was determined at GD 9.5 in WT or L-selectin-deficient mice (n = 15). There were no significant differences between the number of B cells (B220+), T cells (CD3+), or activated granulocytes (Gr-1 high, CD11b+, F4/80+) between CD62L-deficient or WT groups (Figure 2). However, significantly higher (p < 0.05) numbers of NK cells (CD3−LFA1+ Thy 1.2+) were present at the fetal-maternal interface of CD62L-deficient females compared to those observed in WT mice (Figure 2).
3.3. Immunhistochemical Analysis of Leukocytes in GD 9.5 Uterine Samples
Immunohistochemical analysis of GD 9.5 uterine samples supported the flow cytometric data presented in this study and observations previously described by others [11] - [14] . T and B cells were present at low numbers at the fetal-maternal interface and around the yolk sack. Active granulocytes (important effector cells affecting fetal loss or survival) were present at similar levels in both CD62L−/− and WT BALB/c female mice (data not shown). Unfortunately, due to the anatomy of the placenta, it was impossible to assess whether these cells were located intra or extravascularly. NK cells in L-selectin-deficient mice localized primarily to the decidua basalis in greater numbers than observed in WT animals (Figure 3).
4. Discussion
The present study was designed to determine why BALB/c mice genetically deficient for L-selectin delivered significantly higher numbers of viable pups compared to WT controls. To explain this interesting phenomenon, the study focused on identifying the potential immunological differences between WT and L-selectin knock-out mice at their respective implantation sites. Analysis of cell populations at the fetal-maternal interface at GD 9.5 identified significant differences in NK cell numbers between WT and CD62L-deficient BALB/c mice.
L-selectin and its ligands have been shown to play critical roles in the homing, attachment, and tethering of
Figure 2. Uterine leukocyte composition at GD 9.5 in both CD62L−/− and WT BALB/c mice. Uterine samples harvested on GD 9.5 (n = 15) were minced in PBS. Each developing embryo was homogenized in the presence of collagenase D, allowed to digest, labeled with various fluorescent monoclonal antibodies, and analyzed by FACS. Cell groups were defined as follows: NK cells (CD3-LFA1+Thy1.2+); granulocytes (Gr-1+CD11b+F4/80+); B cells (B220+), and T cells (CD3+). Light grey columns represent CD62L-deficient mice and the dark grey bars represent WT animals (*p < 0.05).
Figure 3. Immunohistochemical analysis of the uterus at GD 9.5. Tissues were stained with DBA lectin specific for uterine NK cells (red) and a MECA-32 monoclonal antibody (vascular zone endothelium—green) followed by DAPI staining (nuclei of the trophoblast cells—blue). Samples were analyzed under epifluorescent light microscopy and images overlaid. Uterus at GD 9.5 from WT (A) and CD62L−/− BALB/c mice (B). NK cells (red) localized only at the mesometrial side of the implantation sites (E—embryo), at the decidua basalis (DB), in both images (20× magnification). The DBA positivity reactions were localized to cell surface and to the cytoplasmic granules. Staining intensity reveals accumulation of NK cells in the right image (B). Arrows indicate the exact localization of the cumulating NK cells in both L-selectin ligand deficient and wild type mice, as detected with immunostaining abovementioned.
immune cells to the extracellular matrix of both humans and mice [15] [16] ; however, in the present study migration/trafficking analyses were not performed. Therefore, until a bone marrow transplant between a CD62L−/− donor and a Rag2/γc recipient or between a wild type donor and a Rag2/γc recipient mice is made we will not be able to determine whether immune cell recruitment was higher in CD62L deficient mice. This is the subject of future experiments.
Several previous studies reported that L-selectin−/− mice had a significantly increased total number of splenic lymphocytes (including B and T cells) that comprised up to 30% - 55% of the spleen cell population [17] -[19] . NK cells also localized to the spleen of these mice forming around 12% of all nucleated cells present in the red pulp [20] - [22] . In contrast, no change in the number of either B lymphocytes or NK cells in the has been reported to date in CD62L−/− mice [17] .
NK cells represent approximately 10% of the leukocyte population in both humans and mice [23] . In humans, NK cell subpopulations can be identified based on cell surface expression of CD3, CD16, and CD56; accounting for 3 distinct NK cell subtypes: (1) CD56dimCD16+ (representing about 90% of all NK cells), (2) CD56brightCD16dim, and (3) CD3+CD56+ [24] - [26] . Direct lysis of target cells is the primary effector function for CD56dim NK cells, conversely, effector functions for CD56bright NK cells involves immune regulation [27] . On the other hand, only two populations of NK cells have been described in mice and characterized based on their CD11 (CD11blow and CD11bhigh) expression levels. The CD11bhigh NK cell population can be further categorized into 2 subsets: the CD11bhighCD27high and the CD11bhighCD27low cells [28] . Uterine NK (uNK) cells represent a unique group of NK cells in both species, but their exact place among NK cell types is incompletely understood in mice. In humans, however, uNK cells (CD56bright) can be detected during menstrual cycles in contrast to their mouse analogs that can only be identified by DBA staining after blastocyst implantation [29] .
Using mice lacking lymphocytes (RAG-2−/−), 3 uNK functions were identified as follows: 1) support of terminal decidual cell differentiation, 2) sensitization of spiral arteries resulting in pregnancy-associated dilation and elongation, and 3) formation of a transient lymphoid aggregates at the portal vessels and nerves serving as implantation sites [30] [31] . On the other hand, NK cell-deficient mice remained fertile and delivered normal numbers of viable pups, suggesting that NK cells may not be essential to healthy pregnancies in mice even though significant differences exist between the MLAp (mesometrial lymphoid aggregate of pregnancy) of NK cell-deficient mice and WT animals [32] . Nevertheless, the importance of uNK cells in driving the maturation of uterine spiral arteries into bigger caliber vessels suggested that uNK cells were indeed important to normal pregnancy development since they significantly affected the decidualization and vascularization processes.
Most animal pregnancy models have been designed (by crossing genetically well-defined inbred mouse strains such as C57BL6 and DBA/2) to study mechanisms associated with fetal loss and pregnancy-associated pathologies [13] . This approach thereby mimics the semi-allogeneic graft status of the embryo. In contrast, the present study used an inbred (BALB/c background) colony that allowed us to investigate the specific role of CD62L during pregnancy independent of maternal-paternal MHC gene differences. Although the similarity at the MHC locus in inbred BALB/c mice could eliminate the semi-allogenic graft phenomenon, it could not explain the increase in the number of littermates delivered by CD62L-deficient females.
Based on our observations (and data available in the literature) it is unlikely that NK cells alone accounted for the increase in the number of pups born from CD62L−/− female BALB/c mice. Another possible explanation could be that CD62L-deficient mice presented with alterations in the IL-15 and IFN-γ cytokine signaling pathways [33] [34] (that affect uNK cell proliferation) resulting in a significantly altered micro environment at the fetal-maternal interface favoring fetal development resulting in larger litters. This could occur via different mechanisms, for example, by preventing homing of NK cells into the decidua, affecting their effector functions (making these cells more regulatory in nature), or by preventing pro-uNK cell trafficking from LNs into the pregnant uterus.
5. Conclusion
The increased size in the litters of CD62L−/− BALB/c mice was due to changes affecting female mice. Immunological analyses revealed significantly elevated numbers of NK cells in the uteri of CD62L−/− animals that could have influenced the uterine microenvironment early in pregnancy and played a critical role in regulating maternal tolerance, consequently leading to the delivery of a greater number of viable pups.
Competing Interests
The authors report no conflicts of interest regarding the data presented in this report.
Authors’ Contributions
BF and TTG made substantial contributions to the conception and the design of the study. AM and BF carried out the histopathologic and immunohistochemical analysis and BF also participated in data acquisition and in the pathologic assessment. AA carried out the flow cytometric analysis, mouse breeding, and statistical analysis. JB and FB participated in the design of the study and in drafting the manuscript. KM conceived the study, participated in its design and coordination, helped draft the manuscript, backcrossed CD62L−/− mice into BALB/c background, and provided the animals for the study. All authors read and approved the final version of the manuscript submitted for publication.
Acknowledgements
We wish to thank the staff of the Comparative Research Center at Rush University Medical Center, Chicago, IL, USA. We would like to thank Dr. Oktavia Tarjanyi for her help in the breeding of mice and in the immunostaining procedures. This work was supported in part by the National Institutes of Health Grant (NIH; AR045652), The J.O. Galante Endowment Chair (Rush University Medical Center, Chicago, IL, 60612), and project SROP-4.2.2.A-11/1/KONV-2012-0053 “Investigation of biomarkers in culture medium for the success rate of in vitro fertilization”.
List of Abbreviations
P-selectin - platelet associated selectin
E-selectin - endothelium associated selectin
L-selectin - leukocyte associated selectin
CD62L - leukocyte associated selectin
HEV - high endothelial venules
WT - wild type
mAb - monoclonal antibody
GD - gestational day
NK - natural killer cell
DK - dendritic cell
uNK - uterine natural killer cell
IFN-γ - interferon gamma
CSF - colony stimulating factor
GM-CSF - Granulocyte-macrophage colony-stimulating factor
VEGF - vascular endothelial growth factor
PIGF - placental growth factor
Ang2 - angiopeptin 2
LN - lymph node
DAB - Dolichos Biflorus Agglutinin lectin
NOTES
*Members of the MTA-PTE Human Reproduction Scientific Research Group, Hungarian Academy of Sciences (MTA), Budapest, Hungary.
#Corresponding author.