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The Journal of Neuroscience, February 1, 2000, 20(3):1036-1043
Nitric Oxide Influences Injury-Induced Microglial Migration and Accumulation in the Leech CNS
Aileen Chen1, Shanta M. Kumar2, Christie L. Sahley2, and Kenneth J. Muller1 1 Department of Physiology and Biophysics, University of Miami School of Medicine, Miami, Florida 33136, and 2 Department of Biological Sciences, Purdue University, West Lafayette, Indiana, 47907
ABSTRACT
TOP
ABSTRACT
INTRODUCTION
Damage to the leech or mammalian CNS increases nitric oxide (NO) production and causes accumulation of phagocytic microglial cells at the injury site. The aim of this study was to determine whether NO plays a role in microglial migration and accumulation at lesions in which NO is generated by a rapidly appearing endothelial nitric oxide synthase (eNOS) in leeches. Immunohistochemistry and cytochemistry demonstrated active eNOS before and throughout the period of microglial accumulation at the lesion. Decreasing NO synthesis by application of the NOS inhibitor Nw-nitro-L-arginine methyl ester (1 mM) significantly reduced microglial accumulation, whereas its inactive enantiomer Nw-nitro-D-arginine methyl ester (1 mM) resulted in microglial accumulation similar to that in crushed controls. Increasing NO with the donor spermine NONOate (SPNO) (1 mM) also inhibited accumulation, but not in the presence of the NO scavenger 2-(4-carboxyphenyl)-4,4,5,5-teramethylimidazoline-oxyl-3-oxide (50 µM). The effect of SPNO was reversed by washout. SPNO application reduced average microglial migratory speeds and even reversibly arrested cell movement, as measured in living nerve cords. These results suggest that NO produced at a lesion may be a stop signal for microglia to accumulate there and that it can act on microglia early in their migration. Thus, NO may assume a larger role in nerve repair and recovery from injury by modulating accumulation of microglia, which appear to be important for axonal regeneration.
Key words: nitric oxide; cell migration; endothelial nitric oxide synthase; Hirudo medicinalis; nerve repair; nerve regeneration; microglia
INTRODUCTION
One of the first responses to CNS injury is by microglial cells, the resident macrophages of the brain, which retract their branches, become amoeboid, and migrate to the site of damage. The migration leading to accumulation is thought to be triggered by substances including cytokines released at the damage site, but few studies have examined migration of microglia within the living nervous system. The role of microglia in recovery is controversial, because although they may produce harmful cytotoxins that induce neuronal death (Thanos et al., 1993
; Barron, 1995
Nitric oxide (NO) influences motile cells in both vertebrates and invertebrates. It inhibits migration of rat vascular smooth muscle cells (Sarkar et al., 1996
The injured leech CNS, in which synapse regeneration is successful (Camhi and Macagno, 1991
Portions of this paper have been published previously in abstract form (Chen et al., 1998
MATERIALS AND METHODS
Preparation and operations. Adult 4-6 gm adult leeches (Hirudo medicinalis) were obtained from a commercial supplier (Leeches USA, Westbury, NY) and maintained in artificial pond water (Forty Fathoms, 0.5 gm/l H2O; Marine Enterprises, Towson, MD) at 22°C. For experiments, individual segmental ganglia with connectives or, for time-lapse video microscopy, isolated connectives were dissected in physiological saline (Nicholls and Baylor, 1968
Staining of eNOS and microglial cells. To examine the distribution of eNOS immunoreactivity and microglia at sites of injury, crushed cords were immunostained with monoclonal antibodies to human eNOS (Transduction Laboratories, Lexington, KY), and microglial nuclei then stained with Hoechst 33342 dye. In brief, connectives were dissected, crushed with a pair of fine forceps (Dumont #5), and left at room temperature for 5 min, 3 hr, 6 hr, or 24 hr in L-15. The tissue was then fixed in 4% paraformaldehyde for 20 min, incubated 30 min in a blocking solution [10% (v/v) fetal calf serum and 2% (v/v) Triton X-100 in PBS, pH 7.5], and then kept overnight at 4°C in anti-eNOS monoclonal antibody diluted 1:150 in blocking solution. For the secondary antibody, a 1:200 dilution of Texas Red-conjugated rabbit anti-mouse IgG (heavy and light chain; Molecular Probes, Eugene, OR) was used. The tissue was mounted in glycerol with Hoechst 33342 dye (10 µg/ml) and viewed with a Zeiss (Oberkochen, Germany) epifluorescence microscope and appropriate filters.
Determining the effect of NOS inhibition on accumulation. Microglial accumulation was investigated in the presence of Nw-nitro-L-arginine methyl ester (L-NAME), a general NOS inhibitor. In brief, nerve cords were crushed in a standard manner, incubated in 0.01-1 mM L-NAME or Nw-nitro-D-arginine methyl ester (D-NAME), the inactive enantiomer of L-NAME, in leech saline with 10 mM glucose for 6 hr, fixed 30 min in 4% paraformaldehyde, rinsed in PBS, pH 7.4, and stained 30 min in 1:750 Yo-Pro-1 (Molecular Probes). The Yo-Pro-1 dye was used because it is an argon-ion laser excitable nucleic acid stain that allowed us to view a series of optical sections of washed tissue with a Bio-Rad (Hercules, CA) laser scanning confocal microscope equipped with fluorescein and rhodamine optics and a Nikon (Tokyo, Japan) 20× objective. The accumulation of microglia was analyzed at the crush over an area of ~0.08 mm2, by capturing a Z series consisting of 25 2 µm optical sections through the connectives. For each sample, microglia at the site of injury were counted in every fifth section, and the average number of microglia in the five sections was determined. Statistical significance was determined by ANOVA, followed by post hoc analysis of the significant main effects.
Determining the effect of exogenous NO on accumulation. The NO donor spermine NONOate (SPNO) (Calbiochem, La Jolla, CA) was used to determine the effect of exogenous NO on microglial accumulation. Stock solutions of 100 mM SPNO (100×) were prepared in sodium phosphate buffer, pH 8.5, and stored at
70°C in 10 µl aliquots. Crushed cords were incubated in 1 mM SPNO in L-15 culture medium for 3 hr, and microglial nuclei were labeled with Feulgen's nucleic acid-specific stain, using the method of Morgese et al. (1983)
Once an effect of SPNO on microglial accumulation had been determined, the reversibility of the effect of SPNO was examined. For these experiments, individual ganglia with their attached connectives were dissected intact and placed in L-15 alone (controls) or with 1 mM SPNO. Connectives were crushed by fine forceps anterior and posterior to ganglia and placed in three separate groups. First, as controls, the crushed preparations were incubated in L-15 for 6 hr. Second, crushed preparations were incubated in 1 mM SPNO for 6 hr. Third, to determine whether the effect of SPNO was reversible, a crushed group was incubated 3 hr in SPNO and then washed 3 hr in L-15.
To quantify peak accumulation for each group, the following sampling technique was used with Feulgen-stained tissue, referred to here as a "line count." A hairline in a microscope ocular was positioned perpendicular to the longitudinal axis of the crush, and the number of nuclei within the sheath touching or intersecting the line in a through-focus series at the crush was then counted in a double-blind manner. Counts were made for both connectives at the anterior and posterior margins of the crush in which accumulation was highest, three series each. The counts were averaged and then analyzed using an ANOVA for repeated measures. Post hoc comparisons of the significant effects were assessed with a Newman-Keuls post hoc test. This method measures accumulation at the highest concentration of cells.
Low-light video microscopy. To determine the effect of L-NAME, D-NAME, and SPNO on microglial movement in injured preparations, individual live Hoechst-stained cells were tracked using low-light video microscopy. Procedures were basically those of McGlade-McCulloh et al. (1989)
Movement of microglia in three-dimensional collagen gels. Three-dimensional (3-D) collagen gels (Guthrie and Lumsden, 1994
RESULTS
Nitric oxide synthase and microglial cell accumulation colocalize at sites of CNS injury
To determine the spatial and temporal relationship of injury-induced nitric oxide synthase and accumulating microglial cells, nerve cords were double-stained with a monoclonal antibody for human eNOS and with the fluorescent nuclear dye Hoechst 33342. In uncrushed cords, eNOS immunoreactivity is absent (Shafer et al., 1998
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Figure 1. Appearance of eNOS immunoreactivity and microglial cell accumulation at sites of CNS damage. The connectives connecting ganglia are paired, with the bundled axons of each connective surrounded by a cellular sheath. Adult leech nerve cords were crushed and double-stained with a monoclonal antibody against human eNOS and with the fluorescent nuclear dye Hoechst 33342. The approximate longitudinal extent of the crushes is indicated by vertical dotted lines. Five minutes after crushing, eNOS immunoreactivity was present among nerve fibers in the connectives (A), but microglial cells were still evenly distributed throughout the connectives (B), resembling controls. Note that immunoreactivity was predominantly where crushed axons, glia, and microglia were located and not in the sheath. Three hours after injury, eNOS immunoreactivity persisted at the lesion (C), and microglial cells had accumulated (D). After 24 hr, eNOS immunoreactivity was more diffuse and expanded outside the crush (E). Microglial cells also occupied a larger area (F).
NOS inhibitors block microglial cell accumulation
To determine how NO production at the crush affects microglial cells, NO production was blocked with the NOS inhibitor L-NAME. Microglial cell accumulation in cords was examined 4-6 hr after injury. As controls, crushed cords were incubated in similar concentrations of D-NAME. Microglia accumulated in 1 mM D-NAME (Fig. 2A) but not in 1 mM L-NAME (Fig. 2B). Even at lower concentrations of L-NAME (100-750 µM), accumulation was reduced compared with control cords incubated in leech saline containing 10 mM glucose alone or in D-NAME (data not shown).
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Figure 2. NOS inhibition blocked microglial accumulation. Adult leech nerve cord crushed 6 hr before fixing and stained with the fluorescent nuclear stain Hoechst 33342 to show microglia. Vertical dotted lines indicate longitudinal extent of crush. D-NAME (1 mM), the inactive enantiomer of L-NAME, did not block microglial accumulation at the crush (A), whereas 1 mM L-NAME blocked microglial accumulation (B).
To quantify the effect of NOS inhibition on microglial cell accumulation, microglial cells were counted in a series of planes through the lesion after incubating crushed, living cords 6 hr in L-NAME, D-NAME, or saline vehicle alone. Crushed cords treated with 1 mM L-NAME had counts similar to uncrushed cords, with significantly fewer cells accumulated at the lesion site than crushed controls. In the presence of 1 mM L-NAME, the average ± SEM number of cells accumulated at a crush site was 18.6 ± 1.8 cells, a level similar to noncrushed cords (14.2 ± 1.8), and significantly lower than control cords incubated in saline with glucose (99.8 ± 32.6) or 1 mM D-NAME (105.6 ± 25.3), the inactive enantiomer of L-NAME (n = 4 for each treatment) (Fig. 3). There was a significant difference between the crushed cords treated with 1 mM L-NAME and control cords not exposed to drug treatment (ANOVA; Scheffe's test; F(3,12) = 5.848; p = 0.0106; p < 0.05). Because inhibition of NOS activity reduced the microglial cell accumulation to levels comparable with those in uncrushed cords, it appears that the NO produced after injury influenced the aggregation of microglial cells at the site of injury.
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Figure 3. L-NAME significantly reduced microglial accumulation. In 1 mM L-NAME, significantly fewer cells accumulated at the lesion site than in crushed controls (Crush) and were instead similar to uncrushed controls (data not shown). In contrast, in 1 mM D-NAME, an inactive isoform of L-NAME, microglia accumulated at the crush site in numbers equivalent to crushed control cords. For each sample nerve cord, the average number of microglia at the crush site was determined (see Materials and Methods). There was a significant difference between microglial cell accumulation at the lesion site in injured tissue treated with1 mM L-NAME compared with tissue treated with 1 mM D-NAME (ANOVA; Scheffe's test; F(3,12) = 5.848; p = 0.0106; n = 4).
NO donors block microglial cell accumulation
If microglia aggregate at a lesion as a result of locally increased NO, then a general increase in NO might disrupt the injury-induced NO gradient and interfere with accumulation. Crushed nerve cords were bathed in a 1 mM solution of SPNO, a NO donor with a relatively long half-life (t1/2 = 4 hr at 25°C) for 3 hr, and control cords were bathed in L-15. Control cords incubated in L-15 for 3 hr had large numbers of cells gathered at the lesion (Fig. 4A), whereas cords incubated in the NO donor SPNO had significantly less accumulation there (Fig. 4B). As indicated in Figure 5, control cords incubated in L-15 for 3 hr had large numbers of cells gathered at the lesion (line count, 9.2 ± 0.7 microglia; n = 5 cords), whereas cords incubated in the NO donor SPNO had significantly less accumulation at the crush (4.0 ± 0.4 microglia; n = 3 cords). In cords that were treated with SPNO and then washed, microglia accumulated at the crush (8.0 ± 0.8 microglia; n = 2 cords). No significant differences were observed between the baseline and wash conditions (ANOVA; Scheffe's test; F(2,6) = 20.87; p < 0.002; Newman-Keuls post hoc; p < 0.05).
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Figure 4. NO donor SPNO blocked microglial accumulation. A, Control. Without drug, there was a marked increase in microglia at the lesion (dotted line) inside the sheath by 3 hr. B, Exposure to 1 mM SPNO for 3 hr blocked the accumulation of microglia at the lesion. Cell nuclei were Feulgen-stained.
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Figure 5. Quantitative comparison of the effect of SPNO on microglial accumulation. SPNO inhibited microglial cell accumulation, and this effect was reversible. Nerve cords were crushed and incubated in culture medium (Control) for 6 hr, 1 mM SPNO for 6 hr (SPNO), and 1 mM SPNO for 3 hr followed by a 3 hr wash in L-15 (Wash). Accumulation was measured by counting microglial cell nuclei that intersected a line at right angles to the long axis of the connectives (see Materials and Methods). The SPNO treatment significantly reduced microglial accumulation at the lesion site compared with controls. Washed cords (Wash) had cell counts similar to crush controls that sat for 6 hr in L-15 (Control) but were significantly different from cords that were incubated in 1 mM SPNO for 6 hr (SPNO) (ANOVA; Scheffe's test; F(2,6) = 20.87; p < 0.002; Newman-Keuls post hoc; p < 0.05; n = 5). Error bars are SEM. Groups significantly different from control are indicated by *.
To determine that the effects of SPNO were caused by released NO and not SPNO degradation products, experiments were conducted with aged SPNO, which would have been expected to have a diminished effect. From a single animal, ganglia were exposed 3 hr to 1 mM SPNO depleted by having been prepared 36 hr earlier. With a line count, an average of 5.7 ± 0.2 microglia was measured (n = 8 crushes), which was more cells accumulated at the crush than in segments of cord bathed in fresh SPNO (3.6 ± 0.2 microglia; n = 4 crushes) but was fewer cells than in controls (8.3 ± 0.3; n = 4 crushes). Thus, partially expired SPNO was less potent than a fresh solution in blocking accumulation. Incubation of 1 mM SPNO with 0.5 mM cPTIO, a scavenger of NO in the solution, was sufficient to prevent blocking of microglial cell accumulation (8.0 ± 0.1 microglia; n = 12 crushes). Accumulation of microglia in cPTIO was not different from crushed control cords, showing that cPTIO blocks SPNO inhibition of accumulation and suggesting that the SPNO-induced inhibition of microglial cell accumulation occurred via a mechanism involving NO.
SPNO but not L-NAME blocks microglial cell accumulation by stopping or slowing migration
Video microscopy of living microglia in situ was used to determine why they did not accumulate when NO levels were manipulated. Among the possibilities were that the drug (1) stopped migration, (2) disoriented cells, changing their direction but not rate of movement, or (3) blocked the usual stop signals, causing cells to move through the lesion. With time-lapse video microscopy and low-light fluorescent illumination, live Hoechst-stained microglial nuclei were tracked in crushed connectives (McGlade-McCulloh et al., 1989
Overall, migrating cells stopped or slowed after SPNO exposure; however, a range of behaviors was observed. Figure 6, with each symbol representing a separate cell of six observed, shows the locations of cells at 10 min intervals relative to the start of the treatment period, with positive values representing displacement toward the lesion. Some cells moved toward the crush at variable speeds, even in baseline recordings (top panel). In SPNO (middle panel), the initial responses of cells ranged from immediate stopping (cells 2 and 5) to slowing little (e.g., cell 3). However, toward the end of the SPNO incubation period, all cells slowed if they had not stopped. After washout of SPNO, microglia overall increased their travel (bottom panel). One nucleus (5) initially moved away from the crush, a behavior reported previously for microglia, although for a distance <10 µm, the cell nucleus alone rather than the entire cell might have moved (McGlade-McCulloh et al., 1989
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Figure 6. NO slows migrating microglial cells. The distances traveled by six different microglial cells (indicated by 6 symbols and numbers 1-6 on the abscissa) were measured by low-light fluorescence video microscopy at 10 min intervals for each 30 min treatment period (Baseline, SPNO, Wash). The first point in each plot is time 0. Cells were selected if they could be tracked throughout.
Speed for each cell was calculated from the distance traveled in each 30 min treatment period, and an average velocity was calculated for each treatment group (Fig. 7). For a baseline, mean ± SEM speed was measured to be 0.93 ± 0.13 µm/min (n = 9 cells). For all nine cells, including the six in Figure 6, movement slowed significantly to 0.43 ± 0.12 µm/min during SPNO treatment (p < 0.05), with a recovery to the baseline (0.92 ± 0.07 µm/min) after washout of SPNO. Thus, SPNO blocked microglial cell accumulation by stopping or slowing cells migrating to the crush.
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Figure 7. SPNO slows the migration of cells to a crush. Low-light fluorescence video microscopy was used to track individual Hoechst-stained microglia as they migrated to a crush, as in Figure 6 (n = 9 cells from 2 cords). Selected cells remained in the same focal plane during each 30 min treatment period: baseline (Baseline), 1 mM SPNO (SPNO), and SPNO washout (Wash). A significant decrease in velocity was observed after SPNO exposure (p < 0.05). Cells recovered to baseline velocity after washout. Error bars are SEM. Comparisons were made using Kruskal-Wallis rank sum ANOVA (p = 0.008) and Dunnett's post hoc analysis at the p = 0.05 level.
In contrast to this, slowing of migration caused by SPNO, 1 mM L-NAME, and 1 mM D-NAME did not affect the migration rate of microglia. The average velocity of individual microglial cells in injured nerve cords treated with 1 mM L-NAME was 10.2 ± 2.0 µm/min, whereas the average velocity in tissue treated with 1 mM D-NAME was 8.8 ± 1.4 µm/min. Statistical analysis indicated that treatment with 1 mM L-NAME compared with treatment with L-15 or 1 mM D-NAME did not significantly affect the average velocity of migrating microglia (ANOVA; F(2,18) = 0.434; p = 0.6544; n = 5).
To understand better the mechanisms by which microglia stopped moving in the presence of NO, movement of microglial filopodia and lamellipodia was observed directly in 3-D collagen gels. In gels, the entire cell can be viewed continuously and not only the nucleus in time lapse. Microglia migrated from explants of nerve cord into the gels and were viewed with phase optics for up to 10 d in culture. SPNO, added to a final concentration of 1 mM in L-15 culture medium layered on the gel, completely arrested movement of 10 of 21 cells examined and markedly slowed the movement of nine others, with no effect on two. For 15 cells that had slowed or stopped, washout reversed the effect in nine within the viewing time. An example is shown in Figure 8 in which movement was estimated by subtracting successive frames (top row, difference is white area in last frame). Movement of the lamellipodia stopped with the addition of 1 mM SPNO (Fig. 8, middle row) and resumed within minutes of washout (Fig. 8, bottom row). Addition of aged SPNO solutions as controls had no effect in three preparations examined (data not shown). In two preparations, the NO scavenger reduced-hemoglobin was added either 15 min before addition of SPNO or after incubation in SPNO for 80 min, and in each case, the SPNO was without effect, indicating that NO specifically arrested cell movement.
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Figure 8. NO donor SPNO reversibly arrested movement of microglial cells in three-dimensional collagen gels. Microglia that migrated into the gels moved their lamellipodia with little translocation. Phase contrast images in each row were separated by 5 min intervals; right panels are computer-generated subtractions of the last two images and show cell movement in 5 min in white. Addition of SPNO to a final concentration of 1 mM in L-15 culture medium arrested movement of lamellipodia (middle row), whereas addition of aged NO donor solutions (data not shown) was without effect. The usual motility resumed within minutes of washout (bottom row).
DISCUSSION
NOS activity has been associated previously with the appearance of microglia at CNS lesions in the leech. The present paper demonstrates that microglia accumulate after early expression of NOS activity and eNOS immunoreactivity. Microglia distributed throughout the CNS at the time of injury are one source of NOS activity (Shafer et al., 1998
SPNO acts directly to reduce accumulation of microglia at the lesion by blocking or reducing migration, not through a cytotoxic effect. The inhibitory effect of SPNO was blocked by the NO scavenger carboxy-PTIO, and partially expired SPNO was less effective than fresh SPNO at blocking migration. Aged SPNO might possess toxic NO breakdown products such as peroxynitrites, but these would be expected to increase with time and, if the inhibition were primarily caused by these by-products, then aged SPNO should have enhanced block of accumulation, which it did not. Instead, the blocking effect was reduced, consistent with reduced levels of NO. Third, the effect of SPNO could be reversed by washing either before or after crushing. Both inactive and activated microglia responded to SPNO in a manner inconsistent with cytotoxicity. L-NAME too acted specifically to reduce accumulation, although not by stopping migrating microglia, as the inactive enantiomer D-NAME did not affect accumulation.
Previous work with low-light video microscopy has shown that microglia travel individually to lesions, not moving uniformly as a herd, and that at any time no more than 20% of microglia near a lesion are moving (McGlade-McCulloh et al., 1989
It is possible that the injury-induced NO acts as a stop signal for migrating microglia. According to this hypothesis, the highest concentrations of NO would be at the crush, which would stop the migration of cells, presumably to repair damaged tissue. Both our accumulation and low-light video microscopy studies support this notion. The NO donor SPNO increased NO levels all along the cord, which reversibly arrested migration, even outside the crush. It appears that application of SPNO to the entire cord stopped the cells in place, effectively preventing them from migrating to the crush, resulting in reduced microglial accumulation at the lesion site. Incubation of crushed cords in the NOS inhibitor L-NAME reduced NO levels and microglial cell accumulation but did not affect the migration rate or population of microglia moving. Low-light video recordings in the presence of L-NAME suggest that, in the absence of NO, microglia continue to migrate and do not accumulate at the lesion, supporting the hypothesis that injury-induced NO serves as a stop signal for migrating microglia.
Several substances, including NO, have been shown to inhibit movement or growth at one concentration and have an opposite, promoting effect at other concentrations. In migrating neutrophils, low concentrations of NO can enhance movement and higher concentrations inhibit movement (VanUffelen et al., 1996
The effects of NO on nerve repair and regeneration extend beyond influencing microglia, because NO has been shown to influence the movement of growing axons. In addition to the examples mentioned above, NO halted neurite motility in chick dorsal root ganglion explants (Hess et al., 1993
FOOTNOTES Received Aug. 27, 1999; revised Nov. 8, 1999; accepted Nov. 11, 1999.
This work was supported by National Institutes of Health Grants NS34927 and NS37025 to K.J.M. and C.L.S. We thank Orie Shafer for conducting preliminary experiments, Shirly Mildner for counting microglia, and Susanna Blackshaw for instruction in making collagen gels.
Drs. Chen and Kumar contributed equally to this work.
Correspondence should be addressed to Dr. Kenneth J. Muller, Department of Physiology and Biophysics (R-430), University of Miami School of Medicine, Miami, FL 33136. E-mail: kmuller{at}newssun.med.miami.edu.
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