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The Journal of Neuroscience, August 27, 2003, 23(21):7759-7766
Previous Article | Next Article
Increased Morphological Diversity of Microglia in the Activated Hypothalamic Supraoptic Nucleus
Albert E. Ayoub andA. K. Salm Department of Neurobiology and Anatomy, West Virginia University School of Medicine, Morgantown, West Virginia 26506-9128
Abstract
Top
Abstract
Introduction
Microglia are the immune cells of the CNS. In the normal adult mammalian brain, the majority of these cells is quiescent and exhibits a ramified morphology. Microglia are perhaps best known for their swift transformation to an activated ameboid morphology in response to pathological insults. Here we have observed the responsiveness of these cells to events surrounding the normal activation of neurosecretory neurons in the hypothalamic supraoptic nucleus (SON), a well studied model of structural plasticity in the CNS. Neurons in the SON were activated by substituting 2% saline for drinking water. Brain sections were collected from four experimental groups [controls (C), 2 d-dehydrated (2D), 7 d-dehydrated (D7), and 7 d-dehydrated/21 d-rehydrated animals (R21)] and stained with Isolectin-B4-HRP to visualize microglial cells. Based on morphological criteria, we quantified ramified, hypertrophied, and ameboid microglia using unbiased stereological techniques. Statistical analyses showed significant increases in the number of hypertrophied microglia in the D2 and D7 groups. Moreover, there was a significant increase in the number of ameboid microglia in the D7 group. No changes were seen across conditions in the number of ramified cells, nor did we observe any significant phenotypic changes in a control area of the cingulate gyrus. Hence, increased morphological diversity of microglia was found specifically in the SON and was reversible with the cessation of stimulation. These results indicate that phenotypic plasticity of microglia may be a feature of the normal structural remodeling that accompanies neuronal activation in addition to the activation that accompanies brain pathology.
Key words: plasticity; microglia; SON; hypothalamus; magnocellular neurons; stereology
Introduction
The mammalian CNS is the site of extensive structural plasticity, not only during development but also throughout the lifespan of the organism (Bennett et al., 1964; Greenough, 1988
Despite the large number of studies of astrocytic structural plasticity in the SON, the possible contribution of SON microglia to structural remodeling in this nucleus has received little attention. Generally, microglia are known to serve an immune function and are involved in pathological states (Matsumoto et al., 1992
Some of these data have been presented in preliminary form (Ayoub and Salm, 2000
Materials and Methods
Histochemical staining. Twenty-four adult male Sprague Dawley rats (300-350 gm) of matching age were equally divided into four groups: controls (C), 2 d-dehydrated (D2), 7 d-dehydrated (D7), and 7 d-dehydrated/21 d-rehydrated (R21; n = 6 each group). We induced the activation of MNCs by substitution of 2% saline for drinking water (Jones and Pickering, 1969-D-galactose-containing glycoconjugates on the surface of microglial cells in brain tissue (Streit and Kreutzberg, 1987
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Figure 1. Microglial cells were classified as ramified (A), hypertrophied (B), or ameboid (C). Ramified microglia were defined as having a normal-appearing soma with thin, delicate, and radially projecting processes. Hypertrophied microglia were defined as a having an enlarged, darkened soma and shorter, thicker, and less branched processes. Ameboid microglia were defined as having densely stained, enlarged cell bodies, a few short processes, if any, and often several filopodia. Intermediate morphologies were rare, but excluded from the analysis when encountered. Scale bars, 20 µm.
Stereological analysis. To determine relative SON volumes and quantify microglia, we used an AX70 Olympus (Melville, NY) light microscope, interfaced with a personal computer (Micron PC, ID) and the StereoInvestigator software package (MicroBrightField, Colchester, VT). As determined by StereoInvestigator, we chose four sections through the rostrocaudal extent of the SON by systemic random sampling. This number of sections proved sufficient to provide reliable estimates of relative SON volumes based on an average section thickness of 20-23 µm after histochemical processing. Area measures of the SON included the SON proper containing the magnocellular neurons, plus the underlying dendritic zone and ventral glial limitans. These areas were later used by StereoInvestigator to compute volumes. The number of cells with each of the above morphologies in the SON, and a cortical control area of the cingulate gyrus were then quantified. Before counting, all slides were coded by a colleague to prevent experimenter bias. We used the "Optical Fractionator" method (Bjugn and Gundersen, 1993
Data analysis. GraphPad (San Diego, CA) Prism software was used to analyze parametric data by an ANOVA followed by post hoc Tukey's t test comparisons between groups when appropriate. Bartlett's statistic was used to identify nonparametric data, which was analyzed with a Kruskal-Wallis test followed by Dunn's multiple comparisons.
Results
Volume of the SON
A significant change in the relative volume of the SON (SON proper, plus dendritic zone and underlying ventral glial limitans) was found (F(3,24) = 19.24; p < 0.001) across hydration states. Further comparisons showed that this was caused by a 36% increase in the volume of the D7 group relative to controls (q = 10.04; p < 0.001). SON volumes were as follows: C: 7.8 x 1007 µm3; D2: 8.8 x 1007 µm3; D7: 1.2 x 1008 µm3; and R21: 8.7 x 1007 µm3.Isolectin B4 stains microglial cells in the adult CNS and also has a lower affinity to vascular endothelial cells (Streit and Kreutzberg, 1987
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Figure 2. Representative sections from the SON from control, D2, D7, and R21 experimental groups (top to bottom). At low magnification it can be appreciated that the majority of microglia are in the vicinity of SON capillaries. Microglia were easily distinguished from capillary endothelia at higher magnification (Fig. 4). OT, Optic tract.
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Figure 3. Vascular endothelium in the SON stains slightly with isolectin-B4 (thin arrow). Clearly identifiable ramified microglia (thick arrow) are also visible. Inset, A negative control section pretreated with melibiose does not show stained microglia.
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Figure 4. Example of microglia in the SON taken at high magnification and showing all three phenotypes: carets, ramified; thick arrows, hypertrophied; thin arrow, ameboid; asterisk, blood vessel (images edited with Adobe Photoshop; Adobe Systems Inc., San Jose, CA). Notice extensive filopodia protruding from the ameboid cell in the bottom panel.
Ramified microglia
Ramified microglia were evenly distributed throughout the SON and the brain parenchyma (Fig. 5). The numbers and densities of these cells did not change among experimental groups in the SON (F(3,21) = 0.76; p > 0.05, numbers) (F(3,21) = 0.391; p > 0.05, densities).
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Figure 5. Graphs depicting densities and numbers of microglial phenotypes in the SON across hydration states. n = 6 or 7 in each group. The number of ramified microglia did not show significant change with stimulation. In addition, the density of ramified microglia did not change across hydration states. The number of hypertrophied microglia significantly increased (p < 0.001) in the D2 and D7 groups compared with the control and R21 groups. The density of hypertrophied microglia showed a similar increase. The number of ameboid microglia increased significantly (p < 0.001) in the D7 group compared with the control, D2, and R21 groups. The density of ameboid microglia was also significantly higher in the D7 group, but not in any of the other experimental groups. Error bars indicate SEMs for ramified microglia and minimum-maximum values for hypertrophied and ameboid microglia.
Hypertrophied microglia
Significant changes were observed in the numbers and densities of hypertrophied microglia (H3 = 21.0; p = 0.0001, numbers) (H3 = 20.9; p < 0.0001, densities) (Fig. 5). These changes were apparent, relative to controls by D2 (p < 0.05 both number and density). Further significant increases were seen with prolonged dehydration to D7 (p values <0.001). For both numbers and densities of hypertrophied microglia, no differences were found between controls and the R21 group, indicating that changes in this phenotype were totally reversed with rehydration.Ameboid microglia
Significant changes were also observed in the numbers and densities of ameboid microglia in the activated SON (H3 = 18.3 and 20.8, respectively; p values <0.0001) (Fig. 5). The density, but not the number, of hypertrophied microglia was significantly increased by D2 (p < 0.05) relative to controls. However, the changes from D2 to D7 were robust (p values <0.001, number and density). After prolonged access to normal drinking water after 7 d of saline, there were no differences in numbers or densities of ameboid microglia in the R21 group versus controls. Hence, changes in ameboid microglia were also reversible with the cessation of stimulation.Cingulate cortex
No changes were found in the microglial population in the control area of the cingulate cortex (Fig. 6). Microglia of the cingulate cortex almost exclusively exhibited ramified morphology, and this did not change with hydration state (F(3,21) = 0.39, ramified; 2.19, hypertrophied; 0.66, ameboid: p > 0.05 all cases). Thus, the effect of hydration was localized to the SON and did not affect the control area of the cingulate cortex.
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Figure 6. A, Graphs depicting densities and numbers of microglial phenotypes in the control area of the cingulate cortex across hydration states. An area of the ipsilateral cingulate cortex, of dimensions equal to the SON of that section, was quantified as a per-section-control. As shown in this graph, no significant changes in the density of any phenotype was detected in the area of the cingulate cortex. Error bars indicate SEMs. B, A representative section from a D2 animal showing the control area of the cingulate cortex. The majority of microglia identified in this area had a ramified phenotype in each experimental group.
Total microglia in the SON
To better understand the changes in microglial populations in the SON we also compared total numbers of isolectin-stained microglia in the SON across conditions (Fig. 7a). We found that there was a significant increase in the numbers of microglia (F(3,20) = 7.40; p < 0.002) and that this was not apparent until D7 (q = 6.15; p < 0.01). At this time there was a 37.0% increase in the total number of cells. Again, this change was reversed relative to controls in the R21 group (q = 0.98; p > 0.05).
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Figure 7. A, Graph showing the total numbers of microglia in the SON across hydration state. Significantly more microglia were observed in the SON at D7 (p < 0.01) relative to control and R21. Error bars indicate SEMs. B, Composite graph showing the relative numbers of each microglial phenotype in the SON across hydration states (graph generated using Microsoft Excel; Microsoft Corp., Seattle, WA).
When considered as a percentage of total cells (Fig. 7b), numbers of hypertrophied microglia increased from 1% in controls to 9.3 and 9.7% in D2 and D7 groups, respectively. Numbers of ameboid cells increased from a negligible 0.5% in controls to 11.6% of the total in the D7 group.
Discussion
Here we have shown that consumption of 2% saline instead of drinking water leads to increased morphological diversity of microglia in the SON. This manifests as a significant increase in the hypertrophied phenotype in the D2 and D7 groups and the ameboid phenotype in the D7 group. The changes we observed lasted as long as the dehydration stimulus and reversed with rehydration. Numbers of ramified microglia did not change across hydration state. However, with 7 d of dehydration, there was a significant increase in total microglia. This was accompanied by an overall significant enlargement of the SON at D7. Both of these effects were reversed with rehydration. The reversible increase in relative SON volume was not unexpected because it is known that MNCs hypertrophy when activated (Hatton and Walters, 1973Whether morphological transformation of microglia in the SON is accompanied by the biochemical transformation that microglia undergo in response to brain injury and disease was not addressed in this study. We used isolectin B4 to visualize these cells, because it enabled us to study many more microglia, including ramified microglia that ordinarily do not stain well with antibodies to biochemical markers of activation such as cytokines, CD4, ED1, and MHCII antigens (Flaris et al., 1993
Of interest is the source of increased numbers of hypertrophied and ameboid microglia in the activated SON. Sequential transformation of ramified microglia into hypertrophied and then ameboid phenotypes is likely. This type of transformation occurs in response to disease or peripheral nerve injury (Streit and Graeber, 1993
Another source of increased SON microglia, as well as the selective increases in hypertrophied and ramified forms, may be an infiltration into the nucleus of circulating monocytes. Based on F4/80 labeling, Lawson et al. (1992
Alternatively, those microglia seen astride SON vasculature may belong to the "juxtavascular" population of parenchymal microglia recently studied by Grossmann et al. (2002
From where does the signal leading to morphological transformation (or infiltration) of hypertrophied and ameboid microglia arise? We hypothesized that it might emanate from the CSF in the nearby subarachnoid space, but the absence of microglial changes in the cingulate cortex argues against this possibility. This is also adjacent to the subarachnoid space and has a much thinner glial limitans than does the SON (A. K. Salm, unpublished observations). Therefore the CSF is an unlikely source of any transformation signal, which more than likely originates in the SON instead.
Assuming some SON microglia undergo morphological transformation, it seems plausible that they do so in response to neurotransmitters released in the activated SON. These include GABA, glutamate, noradrenaline, and acetylcholine (for review, see Hatton and Li, 1998
-adrenergic receptors (Fujita et al., 1998
An intriguing possibility is that SON microglia respond to activity-dependent release of interleukin-1
What might be the functional significance of increased microglial diversity in the SON? Clearly the physiologically activated SON is undergoing significant changes, including structural remodeling, increased synaptic activity, and proliferation of endothelia and astrocytes (Murray, 1968
SON microglia may also play a pivotal role in regulating peptides and other substances released in the activated nucleus. Ameboid microglia, increased at D7, provide a source of cytokines such as interleukin 1 (Watt and Hobbs, 2000
Microglial cells are best known for their swift immunoeffector response to pathological states, including autoimmune and other diseases of the CNS and traumatic injuries (Booth and Thomas, 1991
Footnotes
Received Jan 21, 2003; revised July 8, 2003; accepted July 8, 2003.This work was supported by National Science Foundation Grant 9514574.
Correspondence should be addressed to Dr. A. K. Salm, Department of Neurobiology and Anatomy, P. O. Box 9128, West Virginia University School of Medicine, Morgantown, WV 26506-9128. E-mail: asalm{at}hsc.wvu.edu.
Copyright © 2003 Society for Neuroscience 0270-6474/03/237759-08$15.00/0
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