Abstract
Loss of signaling through the endothelin-B receptor (ETB) leads to failure of vagal neural crest (NC) cell colonization of the developing gut and causes congenital distal intestinal aganglionosis [Hirschsprung disease (HSCR)] in humans and other mammals. Several studies suggest that cell–cell interactions and the number of NC cells behind the wavefront may play an important role in successful gut colonization. We compared the number and progression of enteric nervous system stem cells in the wild-type (WT) and HSCR rat gut using whole-mount immunohistochemistry for p75, culture and isolation of NC stem cells (NCSCs) by flow cytometry. Isolation and culture demonstrates that NCSCs enter the WT cecum between embryonic day (E) 13.5 and E14.5, and the number of NCSC in the colon significantly increases after E15.5. These findings are consistent with the caudal progression of the NC-cell wavefront by whole-mount staining. During the period of WT colonic colonization of the proximal colon, we found significant differences in the small bowel NCSC pool between WT and HSCR rats. Whereas the proximal gut NCSC pool in WT rats is increasing behind the colonization wavefront, no such change occurs in the proximal NCSC pool in HSCR rats. Dynamic changes in the NCSC pool occur behind the NC colonization wavefront in the gut of WT rats. The absence of these changes in the HSCR rat may contribute to distal aganglionosis.
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Main
Hirschsprung disease (HSCR) is a congenital abnormality of the enteric nervous system (ENS) and is the most common cause of congenital intestinal obstruction. HSCR is characterized by distal intestinal aganglionosis, and current treatment involves resection of the aganglionic segment of bowel. HSCR affects 1 in every 5000 children born worldwide and is associated with a variety of other congenital anomalies and syndromes. Persistent problems with enterocolitis, diarrhea, constipation, or encopresis are common after resection. Rarely, the length of aganglionic bowel is so great that resection leaves insufficient bowel for nutrient absorption. Morbidity and mortality from this disease remain high, even in developed countries (1).
All of the neurons and glia of the ENS are derived from the neural crest (NC). The majority of enteric ganglia are derived from vagal NC cells that colonize the developing gut in a cranial-to-caudal progression. HSCR occurs when vagal NC cells fail to complete colonization of the distal gut. Several animal models of HSCR exist, and mutations in eight distinct genes are associated with this developmental abnormality in mammals. At least 10% of human HSCR is cause by defective signaling through endothelin-B receptor (ETB) (2). The ETB-null rat is a naturally occurring model of total colonic HSCR (3,4). Postnatally, at least 90% of animals have no ganglion cells beyond the ileocecal junction (3).
Several groups have recently developed techniques to isolate and culture multipotent ENS precursors (5,6). Bixby et al. (6) developed a technique to prospectively identify and isolate enteric NC stem cells (NCSCs) by fluorescence-activated cell sorting (FACS) for high expression of p75, the neurotrophin receptor, and α4 integrin. These cells are self-renewing, comprise only a few percent of fetal gut cells (6), can be identified in the proximal gut of the HSCR rat postnatally, and demonstrate neuronal development after injection into the embryonic distal gut of HSCR rats in organ culture (7). Although it is established that wild-type (WT) gut NCSCs express ETB (8) and the mesenchyme of the developing gut expresses its ligand, endothelin-3, the role of ETB in ENS development at the cellular level remains controversial. An absence of ETB signaling may lead to a primary defect in the ability of NC-derived cells to migrate (7,9) or to a secondary reduction in the ENS progenitor pool through premature differentiation or proliferation failure (10–12).
The colonization behavior of NC-derived cells is influenced by intrinsic factors, molecules expressed by the gut mesenchyme, and interactions between NC cells. The nature and necessity of NC cell–cell interactions in intestinal colonization is just beginning to be examined. Recently, Young et al. (13) demonstrated that when a small population of the most distal hindgut NC-derived cells is isolated from the population behind them, they migrated more slowly. These and similar results support the idea that population pressure behind the wavefront may stimulate distal migration of ENS precursors (14,15). We undertook a series of experiments to examine the localization and dynamics of the gut NCSC population in WT and HSCR rats.
METHODS
Animals.
Protocols were conducted in accordance with National Institutes of Health guidelines and approved and monitored by the University of Michigan University Committee on the Use and Care of Animals. The ETB-null mutation, ETBsl is maintained on an inbred Wistar-Kyoto genetic background. The ETBsl mutation is autosomal recessive. ETBsl/sl rats develop intestinal obstruction in the neonatal period, do not live beyond 36 d, and are referred to as HSCR rats throughout this report. ETB heterozygous rats are indistinguishable from WT rats visually, in lifespan, and in fertility. ETB genotype was determined by PCR analysis of a tail biopsy specimen or, in the case of embryos, from unused portions of the embryo as previously described (16). Embryos were obtained by timed heterozygous mating and killing of the pregnant female rat. Embryos were immediately dissected, with collection of the entire intestine from the esophagogastric junction to the rectum.
Whole-mount immunohistochemistry.
Whole embryonic intestines were fixed in 4% formaldehyde for 3 h at room temperature or overnight at 4°C. After washing with PBS, guts were treated with collagenase (1 mg/mL) for 30 min. The intestines then were incubated for 1 h with 0.5% BSA, 1% DMSO, 0.2% triton-X100, and 5% goat serum in PBS. Rabbit anti-mouse p75 (Chemicon AB1554, Temecula, CA) was added directly to the blocking buffer and incubated at 4°C overnight. After washing with blocking buffer (without goat serum), the intestines were incubated with the secondary antibody, goat anti-rabbit IgG conjugated with HRP (PI-1000; Vector Lab Inc., Burlingame, CA) for 2 h at room temperature. They then were washed with acetate-imidazole buffer (17.5% 1 M sodium acetate and 5% 0.2 M imidazole) followed by Ni-DAB buffer (12.4% 1 M sodium acetate, 5% 0.2 M imidazole, 10% 1 M nickel sulfate, 3% 10 mg/mL diaminobenzidine, and 0.3% of 1% H2O2).
The stained intestines were examined and measured under a dissecting microscope. They were marked into three small intestinal segments of equal length, two cecal segments of equal length, and four large intestinal segments of equal length. The last division of the large bowel is also referred to as rectum. Each section then was individually examined and scored (0–5) for the density of staining in a genotype-blinded manner.
Flow cytometry and cell sorting.
Freshly isolated whole intestines were dissected into cold Ca2+- and Mg2+-free HBSS and divided at the ileocecal junction and just distal to the cecum, forming three segments that are designated in the figures as proximal, cecal, and distal. Intestinal segments were dissociated by incubating for 2 min at 37°C in 0.5 mg/mL deoxyribonuclease I (Sigma Chemical Co.) in Ca2+- and Mg2+-free HBSS. Cells were stained with antibodies against p75 (192I clone) and α4 (Becton-Dickinson, San Jose, CA; Mrα4-1 clone, directly conjugated to phycoerythrin). After washing, cells were resuspended in staining medium that contained 2 μg/mL 7-aminoactinomycin D (7-AAD; Molecular Probes, Eugene, OR). Cell sorting and analysis were performed on a FACSVANTAGE dual-laser flow-cytometer (Becton-Dickinson). Dead cells were eliminated from sorts and analysis as 7-AAD+.
Sorts were performed using two methods for setting the gates. To compare the number of cells with defined levels of expression of p75 and α4 between the two genotypes, we set the gates to collect the top 1% of cells that expressed these markers in the proximal WT gut sections of the same age, stained and sorted on the same day, and all suspended cells were counted. These results are presented in Figs. 3A, 4A, 5A. To address the possibility that ETB deficiency results in a lower level of expression of p75 or α4 without truly affecting the number of multipotent NCSCs, we performed other sorts with the gate set to collect the top 1% of cells that expressed p75 and α4 in the proximal section of that embryo, whether WT or HSCR. This gate resulted in the selection of more cells in HSCR embryos compared with the previously described gate.
Culture of NCSCs.
Cells were cultured as previously described (6). Plates were sequentially coated with 150 μg/mL poly-d-lysine (Biomedical Technologies, Stoughton, MA) and 0.15 mg/mL human fibronectin (Biomedical Technologies) as described (17). Culture plates were kept in sealed plastic bags that contained 6% CO2 before and after sorting to maintain a physiologic pH of the culture medium. Cells were cultured on six-well plates at low density (<30 clones per well). The culture medium was DMEM-low (GIBCO 11885-084) with 15% chick embryo extract, 20 ng/mL recombinant human basic fibroblast growth factor (R&D Systems, Minneapolis, MN), 1% N2 supplement (GIBCO), 2% B27 supplement (GIBCO), 50 μM 2-mercaptoethanol, 110 nM retinoic acid (Sigma Chemical Co.), penicillin/streptomycin (Cambrex BioScience Rockland, Rockland, ME), and 20 ng/mL IGF-1 (R&D Systems). After 6 d, cells were switched to “differentiation” medium, which contains 1% chick embryo extract, 10 ng/mL basic fibroblast growth factor, and no IGF-1. All cultures were maintained in gas-tight chambers (Billups-Rothenberg, Del-Mar, CA) that contained decreased oxygen levels, as previously described (18).
Immunohistochemistry of cultured cells.
Cultures were fixed in acid ethanol (5% glacial acetic acid, 95% ethanol) for 20 min at −20°C, washed, blocked, and triply labeled for Peripherin (Chemicon AB1530) to identify neurons, glial fibrillary acid protein (Sigma Chemical Co. G-3893) to identify glia, and α-smooth muscle actin (Sigma Chemical Co. A-2547) to identify myofibroblasts.
Cell-cycle analysis.
To examine whether the decreased number of NCSCs in the HSCR stomach and small intestine results from decreased proliferation of these cells in vivo, we performed cell-cycle analysis as previously described (19,20). For this experiment, we examined the top 1% of cells that expressed p75 and α4 in the stomach and proximal four fifths of the small intestine. Dissociated gut cells were suspended in medium that contained 5 μg/mL Hoechst 33342 (Sigma Chemical Co.). Cells were incubated in this solution for 45 min at 37°C with agitation every 5–10 min. Cells were kept on ice at all times while stained for flow cytometry analysis.
Statistics.
All results are presented as the mean ± SEM, and p < 0.05 is considered significant. Data were analyzed using GraphPad Prism version 3.00 for Windows (GraphPad Software, San Diego, CA). Comparisons between two groups were made using the nonparametric Mann-Whitney test. Three or more groups were compared using ANOVA.
RESULTS
Localization of NCSCs correlates with vagal NC colonization of the WT rat intestine.
Whole-mount immunohistochemistry for p75 identifies NCSCs, neural progenitors, and mature neurons. We used the technique to identify the NCSC colonization wavefront in WT and HSCR rats. The density and the intensity of the staining were determined on a six-point scale by an observer who was blinded to intestinal location and embryo genotype. Whole-mount staining reveals that cecal colonization by vagal NC cells is well under way at E14.5 in the WT and ETB heterozygous rat but that only the very proximal colon contains NC-derived cells at this time point (Fig. 1A). In contrast, reduced staining was present in the distal small intestine of HSCR embryos compared with WT, and low-density staining was observed only as far distally as the cecum, even at E18.5 (Fig. 1B). Staining in the distal colon of HSCR rats was limited to large extrinsic nerve trunks in the distal colonic segments (Fig. 2).
Next we examined NCSC colonization of the developing rat intestine prospectively by isolation of p75/α4high cells. In WT embryos, we found a cranial-to-caudal progression in the number of p75/α4high cells that correlates well with our whole-mount staining. At E13.5, there is a dramatic increase in the number of p75/α4high cells in the cecal segment. The number of p75/α4high cells begins to rise in the distal segment at E14.5 and reaches its peak at E16.5. It is interesting that in the proximal segment, the number of p75/α4high cells increases after E13.5, behind the p75/α4high colonization wavefront, at peaks at E15.5 (Fig. 3A).
Retrospective identification of NCSCs by culture of unselected, dissociated cells in the WT intestine gives a similar pattern. Although it does not reach statistical significance, the number of NCSCs trends upward in the proximal segment after E13.5. As with prospective sorting, after E13.5, there is a dramatic increase in the number of NCSCs in the cecal segment. This technique does not identify a dramatic increase in distal segment NCSCs until after E16.5 (Fig. 3B).
Culture of selected p75/α4high cells reveals that a high percentage (50–80%) of the resultant colonies were multilineage—that is, they contained cells that stained for neural, glial, and smooth muscle markers. The proximal gut p75/α4high population not only increases in number from E13.5 to E15.5 but also becomes more likely to form multilineage colonies (Fig. 3C).
NCSCs do not colonize the cecum or distal gut of HSCR embryos.
Prospective sorting with a gate set to collect the top 1% of cells that express p75 and α4 in the WT proximal gut section demonstrates no change in the number of p75/α4high cells in the proximal gut of HSCR rats between E13.5 and E17.5 (Fig. 4A). A small number of p75/α4high cells are identified in the cecal and distal gut segments at these time points; however, culture of unselected dissociated gut cells fails to detect significant numbers of NCSC in these gut segments at any time point studied (Fig. 4B).
Culture of p75/α4high cells also fails to yield multilineage colonies (Fig. 4C). These cells were selected using a less restrictive gate (set to collect the top 1% of p75- and α4-expressing cells in the proximal section of the same embryo) to address the possibility that ETB deficiency affects the expression of p75 or α4.
The NCSC pool in the WT but not the HSCR proximal gut increases behind the NC colonization wavefront.
We compared the number of NCSCs in WT and HSCR embryos at different time points in the stomach and small intestine by prospective sorting and retrospectively by culture at clonal density of either dissociated, unselected intestinal cells or selected p75/α4high cells. The number of stomach and small intestinal cells that express high levels of p75 and α4 is reduced in HSCR embryos compared with WT after E14.5, with the most dramatic differences occurring at E14.5 and E15.5 (Fig. 5A). There was no significant difference between the two genotypes in the percentage of p75-positive cells in the p75/α4high gate. Similarly, the number of NCSCs in the proximal gut of WT rats is greater than that of the HSCR rat after E13.5 by unselected culture (Fig. 5B). Culture of selected cells does not reveal this difference until after E14.5 (Fig. 5C). This difference in the percentage of multipotent colonies does not seem to be related to a decreased ability of HSCR p75/α4high cells to survive and form colonies in culture because the difference was observed even in plates with high colony efficiencies, and colony efficiencies were not different between the two genotypes (data not shown).
Culture does not identify altered developmental pathway of cells that express high levels of p75 and α4 in the HSCR intestine.
It is proposed that HSCR occurs in the absence of ETB signaling as a result of increased and premature neuronal differentiation of multipotent ENS precursors. If this is the case, then we might observe altered developmental outcomes in vitro. In addition, the top 1% of p75/α4high gate in the HSCR rat accepts lower levels of expression and, therefore, may select a slightly different population of cells. These cells may be capable of forming only more developmentally restricted colonies in culture. To examine whether the reduced number of multipotent NC-derived cells in the proximal gut of HSCR rats at E15.5 results from restriction of the developmental potential of the selected cells, we analyzed the composition of all colonies derived from the top 1% p75/α4high cells in either genotype in culture. Despite finding reduced numbers of colonies forming all three cell types (neurons, glia, and myofibroblasts), we were unable to identify a difference in the number of colonies that formed only one or two of these cell types between WT and HSCR rats (data not shown). A total of 84 ± 2% of WT p75/α4high cells formed trilineage colonies in culture, whereas only 54 ± 2% of HSCR p75/α4high cells formed trilineage colonies in culture (p = 0.0005; n = 6–8).
Reduced numbers of NCSCs in the stomach and small intestine of HSCR rats is not associated with a generalized reduction in proliferation of these cells.
We examined the cell-cycle distribution in the proximal segment of the developing gut from E13.5 to E17.5. Because we were interested in determining whether there is a generalized proliferation defect in HSCR NCSCs, we removed the last 20% of small intestine from this analysis so that we could compare regions outside the known colonization defect in ETB deficiency. In the stomach and proximal four fifths of the small intestine, we found no difference in the percentage of mitotically active cells using Hoechst 33342 staining of both unselected cells and p75/α4high cells between WT and HSCR rats (Fig. 6). We found a progressive decrease in proliferative activity of these cells between E13.5 and E17.5 in both genotypes.
DISCUSSION
The ability to prospectively identify NCSCs from the developing gut is a powerful research tool and is extremely important in the development of new therapeutic strategies to treat diseases of the ENS. In this study, we detected the maintenance of and regional increases in the NCSC pool behind the colonization wavefront in WT rat embryos. We also compared the dynamics of the NCSC pool between WT rats and HSCR rats and found a significant relative reduction in the HSCR stem cell pool in the small intestine after E13.5—a time when colonization of the rat small intestine seems to be complete.
The original report by Ikadai et al. (3) found that ∼59% of neonatal ETB-deficient rats exhibited aganglionosis proximal to the ileocecal junction, and abnormalities in the small intestinal ENS in postnatal ETB-deficient rats and ET3-deficient mice are reported (21,22). Delayed embryologic development of the small intestinal ENS in HSCR rats is also described (23). Recently, Barlow et al. (24) quantified undifferentiated NC-derived cells in ET3-deficient mouse small intestinal sections using a Phox2B-specific riboprobe. They found an ∼43% reduction in cell number in HSCR sections compared with WT sections at E12.5 but not at E15.5. This is despite the fact that the colonization wavefront had reached the ileocecal junction by E12.5 in ET3-deficient mice and that these mice have normal numbers of myenteric neurons in the ileum postnatally (22). Consistent with our findings in the rat, they concluded that ETB signaling deficiency in the mouse leads to transient reductions in the number and delayed caudal progression of undifferentiated NC-derived cells (24).
Using a FACS gate that selects the top 1% of p75/α4-expressing cells in the WT proximal section, we found a significant reduction in this population in the HSCR rat embryos in the small intestine after E13.5. When we allowed the gate to be defined by each embryo and selected the top 1% of cells that expressed p75 and α4, we found that the selected cells from HSCR stomach and small intestine gut sections were less capable of forming multipotent colonies after E14.5. We suspect that this results from the selection of cells with relatively lower levels of p75 and α4 expression—cells that prove in culture not to be multipotent. Taken together, the decreased number of p75/α4high cells and the reduction in multipotent colony formation in both selected and unselected cultures suggest that HSCR rats have a reduced NCSC pool in the small intestine compared with WT rats after colonization of this region of the gut.
It is interesting that the NCSC pool in the small intestine of WT rats significantly increases between E13.5 and E15.5, when the colonization wavefront is moving through the proximal colon. This raises the issue of the interaction between the number of undifferentiated NC-derived cells in the gut and their ability to migrate. Several studies have shown that reduction in the number of vagal crest cells in vivo reduces the distance that these cells travel in the developing gut (13–15). Young et al. (13) found that if a small population of the most caudal NC-derived cells in the mouse colon is isolated from the population behind them, the cells migrate more slowly. NC-derived cells that were not in contact with other NC-derived cells were immobile in the gut mesenchyme. These findings support the concept that migration may result from “population pressure” behind the leading edge of cells. The development of a large NCSC pool behind the colonization wavefront in WT rats may play a role in the successful colonization of the cecum and proximal colon.
In the mouse, the requirement for ETB activation is restricted to the time when NC-derived cells are colonizing the pericecal region (25,26). This timing and localization are consistent with observations of pronounced abnormal NC cell behavior beginning in the distal small intestine of ET3-deficient mice (27) and with high levels of ET3 expression beginning during this time in the mesenchyme of the developing cecum (24). On the basis of extensive observation of ENS precursor colonization patterns in ET3-deficient and WT mice, Coventry et al. (27) hypothesized that expansion of the pool of undifferentiated NC cells may act as a “driving force” for colonization of the proximal colon. Defects in NC colonization of the ET3-deficient cecum therefore could result from a failure to expand the pool of undifferentiated cells in or proximal to this region.
Sidebotham et al. (28) and Young et al. (29) reported colonization of the entire hindgut in organ culture when segments of proximal gut that contained NC cells were apposed with postcecal colon that lacked NC cells. This may argue against an important role of an expanding NCSC population in the pericecal region for complete hindgut colonization, except that colonization of the hindgut in organ co-culture is significantly different from colonization in vivo. Sidebotham et al. (28) reported that the proximal gut NC cells “demonstrated equivalent ability to migrate to and differentiate in the terminal rectum” as NC cells at the leading edge of colonization in the cecum. However, they noted that the pattern of colonization of the colon in the apposition experiments differed from that of whole gut in vivo and in vitro in that the number of cells was much reduced, the NC cells were largely restricted to the half of the colon adjacent to the site of apposition, and the NC-derived cells predominately migrated superficially around the surface of the apposed terminal rectum with only small numbers of cells penetrating into the mesenchyme (28). Young et al. (29) also noted differences between in vivo colonization of the hindgut by NC cells and colonization in their co-culture experiments. They noted different patterns of marker expression in ENS progenitors in vitro compared with in vivo. They also noted that the growth of cultured gut is considerably less than in vivo. Thus, NC cells that fail to completely colonize the gut in vivo may be able to colonize the hindgut in co-culture because they have less distance to migrate and less gut to colonize than in vivo (29). How well co-culture NC migration experiments reflect the in vivo colonization process is unclear.
The reduction in NCSCs in HSCR rats relative to WT rats may be due to restriction in their developmental potential/premature differentiation, impaired proliferation, or increased apoptosis. The similar percentage of p75-positive cells selected as p75/α4high between the genotypes suggests that the reduction in the number of NCSCs in the HSCR rat is associated with a reduced number of p75-positive cells. This could result from loss of p75 expression with differentiation or a failure in NC cell proliferation. Previous studies have shown unaltered development of NCSCs from the E14.5 whole gut of the HSCR rat compared with WT in culture (7). We obtained similar results when we limited the analysis to just the proximal intestine at E15.5. In vitro differentiation conditions are, of course, extremely different from those encountered by NCSCs in vivo and may not reflect events within the HSCR gut.
We observed a nonsignificant trend for HSCR p75/α4high cells to be less successful in forming colonies over 2 wk in vitro. This suggests a proliferation defect. Barlow et al. (24) examined proliferative activity in undifferentiated ENS progenitors (using SOX10 expression as a marker) from the isolated small bowel of ET3-null mice at E11.5–E12, roughly corresponding to E13.5–E14 in the rat, using short-term culture. They found a significant reduction in the number of proliferating ENS progenitors. However, Woodward et al. (9) examined in situ proliferation of NC-derived cells using bromodeoxyuridine incorporation and found no difference between WT and ET3-deficient mice at E11.5. Whereas the results of Barlow et al. may be an artifact of cell culture, Woodward et al. may have been unable to identify the very small percentage of embryonic gut cells that are undifferentiated ENS progenitors. Using flow cytometry, we detected no difference in in vivo mitotic activity in p75/α4high cells in the stomach and proximal 80% of small intestine. Our data are consistent with the reduction in NCSCs in HCSR stomach and small intestines, being unrelated to changes in proliferative activity of these cells or resulting from very regional (distal 20% of small intestine) differences in proliferation.
We did not examine whether HSCR rat NCSCs undergo apoptosis at increased rates compared with WT rats. Others have looked at this issue and found no increase in apoptosis associated with aganglionosis as a result of deficient ETB signaling (9). However, these studies concentrated on the leading edge of colonization. Increased apoptosis well behind the colonization wavefront may have been missed.
Kruger et al. (7) (including ourselves) used prospective identification of p75/α4high cells to compare the number of NCSCs in the whole gut and identified a 60% reduction in the number of these cells in the HSCR rat compared with the WT rat at E12.5 and E14.5. We proposed that before E12.5 ETB has an effect on NCSC survival or self-renewal that persists but does not worsen with time. Looking prospectively at the isolated small intestine at E13.5, we also identify a reduction (∼43%) in the number of p75/α4high cells. However, culture with retrospective identification of NCSCs suggests that there are equal numbers of NCSCs in the two genotypes at this time point. In addition, in the current work, prospective sorting identified a population of cells in the HSCR cecum and distal colon that were incapable of forming multipotent colonies in culture. Not all cells that are selected on the basis of high p75 and α4 expression are NCSCs. Figure 5C illustrates that 20–50% of the NC-derived colonies formed from these cells are not multipotent. Another possible explanation for the discrepancy between prospectively and retrospectively identified NCSCs in the HSCR rat colon is that our hindgut dissections included sacral crest cells that populate pelvic ganglia in the mesenchyme surrounding the hindgut and are not found in the gut before the arrival of vagal crest cells (at least in the mouse) (30). Because we also found that these cells were incapable of forming multipotent colonies, we would have to speculate that the sorted cells are either not multipotent or that NCSCs that are isolated from this region respond differently to our culture conditions. Bixby et al. (6) found that that NCSCs that were isolated from the rat gut at E14.5 (which would be largely derived from the vagal crest) were more responsive to neurogenic factors than NCSCs that were isolated from the sciatic nerve. Clearly, caution must be used in interpreting the results of prospective identification and quantification of NCSCs without supporting culture data.
The ability to define phenotypically and isolate prospectively the population of enteric NCSCs from postnatal and adult mammals (5,20) suggests the possibility of alternative therapeutic approaches to disorders of the ENS. Several groups have successfully injected undifferentiated NC cells into the fetal gut wall and observed neuronal development in organ culture (7,31). Of course, neuronal and glial development is useless in the absence of functional connections. These connections start early as undifferentiated NC-derived cells migrate in chains along a scaffold created by the processes of leading edge cells (13). Therapeutic creation of a well-functioning ENS may require the induction of embryonic patterns of behavior in a transplanted or persistent NCSC population. Understanding the region-specific patterns of enteric NCSC behavior during normal colonization will aid the development of these new therapeutic approaches.
Abbreviations
- E:
-
embryonic day
- ENS:
-
enteric nervous system
- ETB:
-
endothelin-B receptor
- FACS:
-
fluorescence-activated cell sorting
- HSCR:
-
Hirschsprung disease
- NC:
-
neural crest
- NCSC:
-
neural crest stem cells
- WT:
-
wild-type
- ET3:
-
endothelin 3
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Acknowledgements
We thank Sean Morrison and Genevieve Kruger for help with the isolation and culture of NCSCs, Martin White and David Adams in the University of Michigan Flow Cytometry Core, and Richard Ransom for help in the University of Michigan Department of Pediatrics Imaging Facility.
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Supported by the Wayne Jones Family Fund, The Michigan Gut Peptide Research Center, The Mott Children's Hospital Research Fund
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Tsai, YH., Gariepy, C. Dynamic Changes in the Proximal Gut Neural Crest Stem Cell Population Are Associated with Successful Development of the Distal Enteric Nervous System in Rats. Pediatr Res 58, 636–643 (2005). https://doi.org/10.1203/01.PDR.0000180552.12737.9F
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DOI: https://doi.org/10.1203/01.PDR.0000180552.12737.9F
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