Biochemical and Morphometric Analyses Show that Myelination in the Insulin-like Growth Factor 1 Null Brain Is Proportionate to Its Neuronal Composition

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The Journal of Neuroscience, August 1, 1998, 18(15):5673-5681

Biochemical and Morphometric Analyses Show that Myelination in the Insulin-like Growth Factor 1 Null Brain Is Proportionate to Its Neuronal Composition
Clara M. Cheng¹, George Joncas¹, Rickey R. Reinhardt¹, Robert Farrer², Richard Quarles², Jeremy Janssen¹, Michael P. McDonald³, Jacqueline N. Crawley³, Lynn Powell-Braxton⁴, and Carolyn A. Bondy¹
¹ Developmental Endocrinology Branch, National Institute of Child Health and Human Development, ² Myelin and Brain Development Section, Laboratory of Molecular and Cellular Neurobiology, National Institute of Neurological Diseases and Stroke, ³ Section on Behavioral Neuropharmacology, National Institute of Mental Health, National Institutes of Health, Bethesda, Maryland 20892, and ⁴ Department of Cardiovascular Research, Genentech, San Francisco, California 94080

  ABSTRACT

Top
Abstract
Introduction
Materials & Methods
Results
Discussion
References

To elucidate the role of insulin-like growth factor 1 (IGF1) in the normal development of brain myelination, we used behavioral,biochemical, and histological analyses to compare the myelinationof brains from Igf1^/ and wild-type (WT) littermate mice. The studies were conductedat postnatal day 40, at which time the Igf1^/ mice weighed ~66% less than wild-type mice. However, the Igf1^/ brain weight was only reduced by ~34%. Formal neurological testingshowed no sign of central or peripheral myelinopathy in Igf1^/ mice. Myelin composition was not significantly different, andmyelin concentration, normalized to brain weight or protein, wasequal in Igf1^/ and WT mice. Likewise, concentrations of myelin-specific proteins(MBP, myelin proteolipid protein, MAG, and 2',3'-cyclic nucleotide,3'-phosphodiesterase)were not significantly different in Igf1^/ and WT mice. The myelin-associated lipids galactocerebrosideand sulfatide were modestly reduced in Igf1^/ brains. Regional oligodendrocyte populations and myelin stainingpatterns were comparable in Igf1^/ and WT brains, with the notable exception of the olfactory system.The Igf1^/ olfactory bulb was profoundly reduced in size and was depletedof mitral neurons and oligodendrocytes, and its efferent tractswere depleted of myelin.
In summary, this study shows that myelination of the Igf1^/ brain is proportionate to its neuronal composition. Where projectionneurons are preserved despite the deletion of IGF1, as in thecerebellar system, oligodendrocytes and myelination are indistinguishablefrom wild type. Where projection neurons are depleted, as in theolfactory bulb, oligodendrocytes are also depleted, and myelinationis reduced in proportion to the reduced projection neuron mass.These data make a strong case for the primacy of axonal factors,not including IGF1, in determining oligodendrocyte survival andmyelination.

Key words: IGF1; oligodendrocyte; olfactory bulb; myelin basic protein (MBP); myelin proteolipid protein (PLP); 2',3'-cyclic nucleotide, 3'-phosphodiesterase (CNPase); myelin-associated glycoprotein (MAG)

  INTRODUCTION

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Abstract
Introduction
Materials & Methods
Results
Discussion
References

Insulin-like growth factor 1 (IGF1) and its cognate receptor are highly expressed in the developing brain. IGF1 is selectivelyexpressed in maturing projection neurons of sensory and cerebellarrelay systems during a relatively late phase of their development(Andersson et al., 1988; Ayer-Le Lievre et al., 1991; Bartlettet al., 1991; Bondy, 1991). IGF1 mRNA levels peak during the firstfew weeks of postnatal development and are profoundly reducedin most brain regions, with the exception of the olfactory bulb,after postnatal day 20 (P20) (Bondy, 1991). In response to injury,however, IGF1 gene expression is strongly induced in reactiveastrocytes (Komoly et al., 1992; Lee et al., 1992). IGF1 receptor(IGFR) mRNA is most abundant in IGF1-expressing neurons (Bondyet al., 1992). IGF1 binding sites are coincident with IGFR mRNAin compact nuclear structures and are concentrated in synapticzones adjacent to neurons expressing IGFR mRNA in laminar structures,suggesting that receptors are expressed predominantly on localneural processes (Bohannon et al., 1988, Lesniak et al., 1988).Little IGF binding or IGFR mRNA is detected in white matter (Bohannonet al., 1988; Lesniak et al., 1988; Marks et al., 1991; Bondyet al., 1992). Whereas neurons demonstrate constant or increasinglevels of expression over the course of maturation, IGFR mRNAas a percent of total brain RNA decreases during postnatal development(Werner et al., 1989) because of increasing mRNA contributionfrom neuroglial cells, which express relatively little IGF1 receptor.

The normal developmental timing of IGF1 expression suggests that it is involved in nerve fiber growth, synaptogenesis, and/ormyelination (Bondy, 1991). Recently, in vivo studies of transgenicmice ectopically overexpressing the IGF1 gene during later developmentunder a metallothionein promoter revealed significant increasesin brain size and myelin content (Carson et al., 1993; Ye et al.,1995). An earlier study on IGF1-targeted gene deletion (Igf1^/) brains reported hypomyelination based on a decrease in the sizeof anterior forebrain myelin tracts but did not investigate myelinationin other brain regions or in the brain as a whole (Beck et al.,1995). To further examine the role of IGF1 in brain myelination,in the present study we have used biochemical, histological, andbehavioral analyses to evaluate all aspects of myelination ona whole-brain and region-specific basis in the Igf1^/ mouse brain using postnatal day 40 (P40) Igf1^/ and wild-type (WT) littermates. At this age, myelination of themouse brain is essentially complete (Morell et al., 1972; Matthieuet al., 1973).

  MATERIALS AND METHODS

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Abstract
Introduction
Materials & Methods
Results
Discussion
References

Animal tissue. The Igf1^/ mouse line used in this study, which had been bred into a CD1 inbred line for more than six generations,was approved by the National Institute of Child Health and HumanDevelopment Animal Use and Care Committee and was generated atGenentech, Inc. (San Francisco, CA) (Powell-Braxton et al., 1993).Igf1^/ and WT littermate mice were genotyped as described previously(Powell-Braxton et al., 1993) and killed by decapitation at P40for experimental comparison. For biochemical analysis and frozensection preparation, brains were removed, snap frozen, and storedat $-$ 70°C until used. Sections 10 µm thick were cut sagittallyat $-$ 20°C, thaw-mounted onto poly-L-lysine-coated slides, and storedat $-$ 70°C.

Myelin isolation. Brain myelin was isolated by sucrose density gradient centrifugation as described by Quarles et al. (1985).Briefly, brains were homogenized in 0.32 M sucrose (1 gm/20 ml)and layered over an equal volume of 0.85 M sucrose. After centrifugingat 75,000 × g for 30 min, myelin was collected from the interfaceand osmotically shocked with water on ice for 30 min. The largemyelin fragments were sedimented at 12,000 × g for 20 min, resuspendedin a buffer containing 10 mM Tris-HCl, pH 8.0, and 1 mM EDTA forprotein concentration determination by the method of Bradford(1976).

Immunoblotting. Protein (25 mg) from total brain homogenate or myelin fractions was loaded on precast 4-20% SDS-polyacrylamidegels (Novex, San Diego, CA) and transferred to nitrocellulosemembranes using an electrophoretic transfer cell (Bio-Rad, Hercules,CA). The primary antibodies used for immunoblotting were obtainedfrom the following sources: anti-2',3'-cyclic nucleotide,3'-phosphodiesterase(CNPase) (1:400) and anti-myelin proteolipid protein (PLP) (1:250)from Chemicon (Temecula, CA); anti-myelin basic protein (MBP)(1:1000) from Sternberger Monoclonals (Baltimore, MD); and B11F7anti-myelin-associated glycoprotein (MAG) monoclonal antibodyas previously described (Doberson et al., 1985). After incubationwith horseradish peroxidase-linked secondary antibodies, proteinbands were visualized on Kodak (Rochester, NY) XAR film by ECLdetection reagents (Amersham, Cleveland, OH). A digital imageof the immunoblots was made, and the relative amounts of myelin-specificproteins in WT and Igf1^/ samples were compared using the NIH Image 1.57 program.

Immunohistochemistry. Immunohistochemistry was performed by the avidin-biotin-immunoperoxidase method. Briefly, frozen brainsections were fixed in 4% formaldehyde for 10 min, quenched in3% H₂O₂ for 10 min, and then blocked in 10% normal serum for 30min, followed by incubation overnight at 4°C with primary antibodies.The anti-MAG antibody was as described above, and the anti-PLPwas purchased from Biogenesis (Sandown, NH). These antibodieswere used at dilutions of 1:100 and 1:50, respectively. Sectionswere incubated with biotinylated secondary antibodies (1:400)for 30 min. The signal was detected and amplified using the ABCperoxidase method (Vector Laboratories, Burlingame, CA), and visualizedwith 3,3'-diaminobenzidine. Sections were counterstained withmethyl green.

Lipid analysis. Total brain homogenates prepared as described for myelin isolation were centrifuged at 100,000 × g for 1 hr.Pellets were resuspended in water and centrifuged again at 100,000× g for another hour. Resulting pellets, considered as total membranefraction, were suspended in water, and lipids were extracted withchloroform/methanol (C/M; 1:1, v/v) so that the final ratio ofchloroform/methanol/water was 5:5:1. Neutral glycosphingolipidsand sulfatide were separated from gangliosides by a modificationof the phase partitioning method originally described by Folchet al. (1957). The C/M extract was adjusted to a ratio of 2:1(C/M, v/v) with the addition of chloroform, and aqueous and organicphases were generated by adding 0.74% KCl. The lower organic phasewas subjected to mild alkaline methanolysis to destroy alkali-labileglycerophospholipids. The lower phase glycosphingolipid fractionsrepresenting equal amounts of protein were chromatographed on10 cm silica gel 60 high performance thin layer chromatography(HPTLC) plates (Merck, Darmstadt, Germany) in chloroform/methanol/water(65:25:4). Glycolipids were detected with Orcinol reagent, andgalactocerebroside and sulfatide were identified by their comigrationwith standards. A digital image of the orcinol-stained HPTLC platewas made, and the relative amounts of galactocerebroside and sulfatidein WT and IGF1 null samples were compared using the NIH Imageprogram.

Luxol fast blue-periodic acid Schiff-hematoxylin stain. For histological staining of myelin sheaths, frozen brain sectionswere fixed in 4% formaldehyde, stained in 0.1% Luxol blue at 60°Covernight, and differentiated in 0.05% lithium carbonate for 30sec, followed by 70% ethanol for 10 sec (Margolis and Pickett,1956). After rinsing in distilled water, sections were oxidizedin 0.5% periodic acid and then stained in 0.5% Schiff's solutionfor 15 min. Sections were finally counterstained with hematoxylin.

In situ hybridization. In situ hybridization was performed as described previously (Bondy and Lightman, 1989), and oligomersequences of PLP and MBP used for probe synthesis were as describedby Komoly et al. (1992).

Morphometry. The area of whole-brain sections and structures, including the olfactory bulb, anterior commissure (AC), andcerebellum, was measured using computerized image analysis. Anatomicallymatched sagittal sections were digitized using a solid-state videocamera. The structures were outlined by cursor control, and theareas were obtained in pixels using the NIH Image program (seeabove). The width of cerebellar medullary ray forming the stalkof the four and five lobules at the level of the origin of thepreculminate and primary fissures was measured on micrographstaken at 200×. Two to four independent measurements per animalwere obtained for each structure. The evaluation of cell densityand PLP mRNA-positive cell density was done manually with a microscopeat 200-400× and on micrographs taken at the same magnifications.PLP mRNA-positive cells were defined as having at least five exposedsilver grains.

Neurological testing. Thirty mice (14 WT and 16 Igf1^/) were used for behavioral testing. Mice were 35-45 d old at the startof testing. Weights were recorded at the time of testing to facilitateanalysis of data by size as well as genotype differences. Forgeneral neurological function, a battery of tests was performedas described previously (Irwin, 1968; Crawley and Paylor, 1997),including righting, air-righting, whisker-orienting, eye blink,pinna twitch, and Preyer auditory reflexes, as well as reachingresponse and response to an approaching object. Rotorod performancewas tested as described by Liu et al. (1997), and wire-hang latencywas measured according to the method of Sango et al. (1996).

  RESULTS

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Abstract
Introduction
Materials & Methods
Results
Discussion
References

Myelin content

At P40, Igf1^/ mice weigh ~66% less than WT littermates (8.92 ± 1.27 vs 25.98 ± 1.79 gm; n = 6 for each group). Igf1^/ brain weight, however, is only reduced by approximately one-third(Table 1). Myelin is decreased by 37% in the Igf1^/ brain compared with the WT, in parallel with the reduction inbrain size (Table 1). When myelin is normalized to brain weight,there is no significant difference between Igf1^/ (5.52 ± 0.50 µg myelin/mg brain) and wild type (5.77 ± 0.56 µgmyelin/mg brain). Similar results were obtained when the datawere expressed as micrograms of myelin per milligrams of totalbrain protein (Table 1). Thus, total myelin content in the Igf1^/ brain is reduced in proportion to brain size, and myelin concentrationis equivalent in Igf1^/ and WT brains.


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Table 1. Comparison of brain weight, protein, and myelin content in Igf1^/ mice and wild-type littermates

Myelin proteins

The expression of the major myelin proteins was compared in both total protein preparations and purified myelin fractions(Fig. 1). MAG, MBP, PLP, and CNPase levels were equal in myelinfractions from Igf1^/ and WT brains (Fig. 1B). In total protein blots, MAG and MBPwere reduced by ~15% in Igf1^/ brains, but this difference was not statistically significant(Fig. 1B).

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Figure 1. Immunoblot analysis of myelin-specific proteins in Igf1^/ (Null) and wild-type (WT) brains. A, Representative immunoblots of myelin fraction proteins isolated by sucrose density gradient centrifugation and separated on 4-20% polyacrylamide gels. The proteins were blotted onto nitrocellulose membranes and probed with antibodies against MAG, MBP (left), CNPase, and PLP (right). The bands representing these proteins are marked by arrows and appear at the positions of expected molecular weight: MAG, 100 kDa; MBP, 14, 17, 18, and 21.5 kDa; CNPase, 48 kDa; PLP, 25 kDa. These blots show data from three WT and three Igf1^/ mice; similar results were obtained with additional groups. B, Quantitation of CNPase, PLP, MAG, and MBP levels determined by immunoblotting of total brain protein and brain myelin fractions. Protein bands from the blots shown in A and blots from other independent trials were quantified using computer-assisted image analysis. Data are expressed as mean ± SEM of percentage of WT values (n = 6 for both WT and Igf1^/ groups). None of the values represents a significant difference between Igf1^/ and wild type.

Cellular patterns of PLP and MAG protein localization were evaluated by immunohistochemistry. Figure 2 shows very similarintensity and distribution of PLP immunoreactivity in white mattertracts of WT and Igf1^/ mice. Parallel sections probed with anti-MAG antibody also revealedno evidence of a decrease in MAG intensity or altered distributionin Igf1^/ brains (data not shown). In situ hybridization histochemistrycomparing regional PLP and MBP gene expression in WT and Igf1^/ brains reveals virtually identical neuroanatomical patterns ofexpression (Fig. 3), except for a substantial reduction in bothtranscripts in the Igf1^/ olfactory bulb (see below).

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Figure 2. Immunohistochemical comparison of the regional expression of PLP in WT (A, C) and Igf1^/ brains (B, D). Anatomically matched sagittal P40 brain sections were probed by anti-PLP antibodies visualized with 3,3'-diaminobenzidine (brown) and counterstained with methyl green. Micrographs show the homogeneous distribution of PLP in myelinated tracts of the cerebellum (A, B) and striatum (C, D). cc, Corpus callosum; f, fimbria. Scale bar, 200 µm.

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Figure 3. Comparison of PLP and MBP gene expression in the anterior forebrain and cerebellum of wild-type (WT, left panels) and Igf1^/ mice (Null, right panels) by in situ hybridization. Serial sagittal brain sections of WT and Igf1^/ brains were hybridized to ³⁵S-labeled oligomer probes for MBP (A, B, E, F) and PLP (C, D, G, H). Dark-field micrographs show the hybridization signal as white grains. ac, Anterior commissure; cc, corpus callosum; f, fimbria; HI, hippocampal formation; IC, inferior colliculus; med, cerebellar medulla; TH, thalamus. Scale bar, 400 µm.

Myelin lipids

Characteristic lipid components of myelin were compared by thin-layer chromatography (Fig. 4). Galactocerebroside and sulfatidelevels per milligram of total protein were reduced by ~25% inthe Igf1^/ brains. Luxol blue histochemical staining was used to assessmyelin concentration in specific brain regions (Fig. 5). The anteriorlimb of the anterior commissure (al/AC) and the olfactory tractdemonstrated a profound reduction in Luxol staining in Igf1^/ brains compared with wild type (Fig. 5A-D), in contrast to theessentially normal pattern of staining obtained in other brainstructures, e.g., the cerebellum (Fig. 5E,F). The anterior limbconsists of axons originating from the olfactory bulb, which isunique among brain structures in demonstrating continued highlevels of IGF1 expression during adulthood (Bondy, 1991).

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Figure 4. Myelin lipids in WT and Igf1^/ brains extracted from equal amounts of total protein demonstrated by thin layer chromatography. Orcinol-stained bands are identified as galactocerebroside (Gal C) or sulfatide (Sulf) by comparison of the comigrating standards (St) in A. The bands were quantified by the NIH Image analysis program, and the results are expressed as mean ± SEM of percentage of wild type (B).

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Figure 5. Luxol blue myelin staining in WT (A, C, E) and Igf1^/ (B, D, F) brains. A and B show the olfactory tract (ot) leading into the olfactory bulb at low magnification. The anterior and posterior limbs (al and pl, respectively) of the AC are seen on the left side of A and B. C and D show ACs at higher magnification at a medial level in which two limbs have joined, showing that the anterior limb is deeply stained in the wild type but very faintly stained in the Igf1^/. E and F compare Luxol staining in the cerebellum. The lipophilic Luxol stain is marine blue, and hematoxylin-stained nuclei are navy blue. Scale bar: A, B, E, F, 400 µm; C, D, 50 µm; E, F, 200 µm.

Regional morphometry and oligodendrocyte distribution

Given the marked reduction in size and myelin staining of the al/AC, we compared the size of the olfactory bulb and otherbrain structures, such as the cerebellum, where myelination appearsnormal. The olfactory bulb was reduced in area by 60%, whereasthe whole-brain section and cerebellar areas were reduced by only25-30% in Igf1^/ compared with WT brains (Table 2). The projection neurons ofthe Igf1^/ cerebellar cortex were significantly increased in density suchthat their total number is probably equal in WT and Igf1^/ brains, whereas mitral neuron density was not increased in theIgf1^/ olfactory bulb (Table 2), suggesting at least a 60% reductionin the number of olfactory projection neurons, given the 60% decreasein olfactory size.


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Table 2. Regional morphometric analyses

Oligodendrocyte populations were evaluated by counting PLP mRNA-positive (PLP+) cells in terms of number per area and as apercentage of all cells in a given area. PLP+ cells were increasedin density in the Igf1^/ cerebellum and posterior limb of the AC, but their numbers wereequal or reduced in the anterior limb of the AC and olfactorybulb (Fig. 6, Table 2). The reduction was most pronounced inthe external plexiform layer but was also significant in the mitralcell layer (Fig. 6A-D, Table 2).

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Figure 6. Oligodendrocyte concentration in olfactory bulb (A-D) and cerebellar medulla (E-H). PLP mRNA-positive cells are taken to be oligodendrocytes. In this figure, each bright-field micrograph is paired with a matching dark-field illumination showing the PLP mRNA-positive cells. The wild-type (WT) olfactory bulb (A, B) is much larger than that of the Igf1^/ (Null) (C, D). The number of mitral neurons and PLP mRNA-positive cells are both reduced in the Igf1^/. ep, External plexiform layer; ig, internal granular layer; ip, internal plexiform layer; m, mitral cell layer; ot, olfactory tract. PLP mRNA-positive cells are shown at higher magnification on the cerebellar medulla of WT (E, F) and Igf1^/ (G, H) brain sections. Scale bar: A-D, 200 µm; E-H, 50 µm.

Neurological function

All reflexes and measures of gross sensory function were normal in Igf1^/ mice. Igf1^/ mice performed better than wild types on the wire-hanging latencytest, which measures neuromuscular function and grip strength(this may be partially explained by their lesser weight, becausesmaller mice tend to perform better on this test), whereas therewas an ~30% decrease in rotorod performance for the Igf1^/ mice (Table 3). Evaluation of gait by comparing paw print tracingsshowed no abnormality in the Igf1^/ mice, with shorter distances between steps proportionate to theirreduced size (data not shown).


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Table 3. Neurological testing of Igf^/ mice and wild-type littermates

  DISCUSSION

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Abstract
Introduction
Materials & Methods
Results
Discussion
References

This study shows that brain myelin is proportionate to brain mass in Igf1^/ mice and that these mice show no overt behavioral signs of dysmyelination,suggesting that myelination is not significantly impaired despiteIGF1 deletion. The proportionate reduction in myelin content,demonstrated by equivalent whole-brain myelin concentrations,is likely explained by the reduced dimensions of neuronal processesin these dwarf mice, and in some cases, e.g., the olfactory bulb,by the depletion of neurons. In brain structures in which theprojection neurons are preserved, oligodendrocyte numbers andmyelination are preserved in WT and Igf1^/ mice, despite the loss of IGF1, but in structures where the projectionneurons are depleted, oligodendrocyte numbers and myelin stainingare selectively diminished, suggesting a primary role for neuralfactors other than IGF1 in oligodendrocyte survival and myelination.The present findings are consistent with the neurological phenotypeof an Igf1^/ man who is severely mentally retarded but who shows no evidenceof dysmyelination (Woods et al., 1996). Furthermore, these datasuggesting a primary neuronal function for IGF1 in brain developmentagree with the primarily neuronal patterns of IGF1 and IGFR expressionduring brain development (Bondy and Lee, 1993).

Beck et al. (1995), in a previous study of the Igf1^/ brain, reported that IGF1 gene disruption resulted in brain hypomyelination.This conclusion was based primarily on the observation of an apparentlydisproportionate reduction in size of white matter tracts in theanterior forebrain. Using anterior coronal sections to evaluatemyelination, they found an ~70% reduction in AC area and medialcorpus callosum thickness. Given that whole-brain size was reducedby only one-third, it was concluded that there was a selectivereduction in myelination affecting the Igf1^/ brain. However, that study did not assess myelination in otherbrain areas or the brain as a whole and did not investigate theneural structures giving rise to the affected forebrain myelintracts. In contrast, the present study used an integrated whole-brainapproach to the evaluation of myelination in the Igf1^/ brain. We examined neuroanatomical patterns of myelination inthe Igf1^/ mouse from brainstem to olfactory bulb and found that white matterstructures were proportionate in size to relevant neuronal structures.The brain as a whole and most component structures were reducedin size by approximately one-third compared with wild type, andmyelination was reduced in a parallel manner.

Throughout most of the Igf1^/ brain, cell density is increased (Beck et al., 1995; present study), suggesting that much of thedecrease in brain size is attributable to decreased neuropil.For example, the cerebellum is reduced in area by 30%, but Purkinjecells and oligodendrocytes are increased in density, such thattheir total numbers may be very similar in WT and Igf1^/ cerebella. Myelination, in terms of the size of cerebellar whitematter tracts and intensity of staining for myelin and myelin-specificproteins, appears quite normal throughout the Igf1^/ cerebellum, despite the fact that IGF1 is normally highly expressedby inferior olivary, Purkinje, and deep cerebellar projectionneurons during development (Bondy, 1991). This observation suggeststhat if the system projection neurons survive despite the lackof IGF1, oligodendrocytes survive and appropriate myelinationoccurs. The Igf1^/ olfactory bulb, in contrast to the cerebellum, was reduced insize by 60% and had a reduced number of projection neurons andoligodendrocytes. Central olfactory white matter tracts were correspondinglyreduced in size by 60%. Our study thus confirms the marked reductionin the size and myelin staining of the anterior limb of the ACas noted by Beck et al. (1995), but shows that this defect relatesto olfactory neural hypoplasia, rather than being emblematic ofa generalized defect in myelination. Together, the observationsin cerebellum and olfactory bulb suggest that oligodendrocytesurvival and myelination are determined by neural factors otherthan IGF1.

The anterior limb of the AC consists of olfactory axons crossing to the contralateral olfactory cortex, whereas the posteriorlimb comprises decussating temporal lobe axons. The present studyshows markedly reduced myelin staining in the anterior but notposterior limb of the Igf1^/ AC, indicative of a selective impairment of the olfactory component.As a possible explanation for this marked defect in the Igf1^/ olfactory system, we note that mitral neurons normally expressIGF1 throughout life, suggesting a sustained and apparently criticaldependency on this anabolic peptide, in contrast to other systemsin which projection neurons demonstrate transient IGF1 expressionduring development (Bondy, 1991). The reduced axon number in theAC (Beck et al., 1995) stems from the reduced number of mitralcells in the hypoplastic Igf1^/ olfactory bulb, and the reduced myelination of remaining axonsprobably reflects an attenuation in size or electrical activityof axons arising from IGF1-deficient olfactory projection neurons.Substantial evidence indicates that oligodendrocyte survival andmyelin sheath formation are linked to axonal contact, with largeror more active axons stimulating more oligodendrocytes to surviveand produce more extensive myelination (Barres et al., 1992, 1993;Barres and Raff, 1993). By analogy with the winnowing of peripheralnerves to match the size of target zones, the axon appears tobe the target zone of oligodendrocytes, whose number is thus appropriatelymatched to specific axonal myelin needs.

Beck et al. (1995) also noted a reduction in vertical diameter, or thickness of the medial limb of the corpus callosum. Thecorpus callosum is more heterogeneous than the AC, consistingof populations of crossing cortical axons, which vary at eachrostrocaudal and mediolateral plane, making it difficult to knowto which specific neuronal subpopulation its size should be comparedat any given level. It is possible that their measurements includedthe hippocampal commissure underlying the corpus callosum. Thisstructure, containing crossing dentate gyrus axons, should reflectthe disproportionate reduction in size of the dentate gyrus, notedby the same authors (Beck et al., 1995). The fact that on a whole-brainbasis myelin and myelin-specific protein concentrations are equalin WT and Igf1^/ brains suggests that the attenuation of the corpus callosum isproportional to a corresponding diminution in neural mass. Supportingthis view, a recent analysis of the peripheral nervous systemin Igf1^/ mice showed reduced axonal diameter with myelination proportionateto axon size and no evidence of peripheral myelinopathy (Gao etal., 1997).

The view that myelination in Igf1^/ mice is essentially matched to neural mass and presumably needs is supported by functionaldata. Primary myelin deficiencies are associated with neurologicalconsequences, including tremor and impaired motor skills and coordination,whereas Igf1^/ mice demonstrate normal or modestly impaired neuromuscular functions.Further support for the view that IGF1 is not primarily involvedin myelination is provided by the finding that a young man nullizygousfor Igf1 is mentally retarded but does not have any signs of dysmyelinationon clinical examination or brain imaging (Woods et al., 1996).

The idea that IGF1 had a role in brain myelination began with in vitro studies showing that IGF1 promotes oligodendrocyteproliferation, survival, and differentiation (for review, seeMcMorris and McKinnon, 1996). However, the present study showsthat, with the exception of the olfactory bulb (in which projectionneurons are also depleted), oligodendrocyte numbers and differentiationare not deficient in the Igf1^/ brain, demonstrating that IGF1 does not have an essential orgeneralized role in oligodendrocyte development in vivo. It couldbe argued that the role of IGF1 is taken over by IGF2 in the Igf1^/ brain, because IGF1 and IGF2 both activate the IGF1 receptorand IGF2 is expressed in brain. However, the entirely differentdevelopmental regulation and spatiotemporal patterns of expressionof these two peptides (Bondy et al., 1992) make it difficult toimagine interchangeable actions in brain development. The "redundancy"rationalization is particularly unconvincing, because the Igf1^/ brain has multiple defects that are clearly not compensated byIGF2, including the olfactory bulb hypoplasia noted in the presentstudy, as well as selective deficits in dentate gyrus granulecells and in a subpopulation of striatal neurons, as demonstratedby Beck et al. (1995).

The fact that IGF1 does not seem to have a major role in developmental myelination does not mean that it is not importantin repair processes called into play after nervous system injury.IGF1 expression is induced in reactive astrocytes responding toischemia (Lee et al., 1992) and demyelinating insults (Komolyet al., 1992), and IGFR expression is enhanced in injured oligodendrocytes(Komoly et al., 1992), and administration of exogenous IGF1 improvesremyelination after injury (Yao et al., 1995). The prominent effectsof IGF1 on oligodendrocytes in vitro may actually be explainedby the fact that culture is essentially an injury model system,with the cells struggling to survive and function after traumain adverse conditions, deprived of their normal nurturing environment.

Observations in transgenic mice overexpressing IGF1 under the control of a metallothionein promoter have been invoked to supporta primary role for IGF1 in myelination (Carson et al., 1993).This model involves the ectopic expression of IGF1 from unidentifiedbrain cells during a relatively late phase of development afternormal endogenous IGF1 expression has subsided (except for theolfactory bulb). Both brain size and myelin content are increasedin the transgenic, but DNA content and oligodendrocyte numbersare not, so it appears that the increased brain mass is attributableprimarily to increased cell size and/or process growth. A recentinvestigation of this transgenic model (Ye et al., 1995) showedthat axonal diameter is significantly increased in IGF1-overexpressingbrains and that myelin sheath thickness correlates positivelywith axonal diameter. If, as discussed above, myelination is inducedby neuronal fiber growth and/or activity, then a straightforwardexplanation for the findings in the transgenic model is that IGF1overexpression late in development stimulates excessive growthin size and/or activity of axons (and possibly dendrites), which,in turn, stimulates additional oligodendrocyte biosynthetic activityand myelination.

The view that the primary effects of IGF1 are on neurons reflects the normal in vivo patterns of IGF1 and IGFR expression,which are primarily neuronal. For example, in the olfactory bulb,IGF1 is expressed by mitral and tufted neurons (Bondy, 1991),and the IGFR is concentrated in the glomerular, plexiform, andmitral layers but not in the olfactory nerve or tract (Wertheret al., 1989; Marks et al., 1991). The most likely scenario isthat IGF1, released locally from olfactory projection neuron somaand dendrites, acts in an autocrine or paracrine manner on theprojection neurons, enhancing their survival, growth, and activity.In the absence of IGF1, fewer projection neurons survive, andthose that do are asthenic. As a secondary result of this neuraxonaldeficiency, oligodendrocytes are reduced in number and make lessmyelin, perhaps attributable to loss of axonal factors that normallystimulate oligodendrocytes. This is not likely to include IGF1,because IGFR expression is not normally detected in these neuroglialcells in vivo and because there seems to be no problem with oligodendrocytesurvival or myelination in other brain structures, such as thecerebellum, in which the projection neurons survive despite thelack of IGF1. Thus, the data from studies in the Igf1^/ brain and the IGF1 overexpression brain are best explained bythe simple hypothesis that IGF1 stimulates neuronal process growth,which in turn stimulates myelin formation.

In summary, in this study we show that myelination of the Igf1^/ brain is proportionate to its neuronal composition whether analyzedon a region-by-region or whole-brain basis. We show that whereprojection neurons are preserved, as in the cerebellar system,oligodendrocytes and myelination are robust and indistinguishablefrom wild type. Where projection neurons are depleted, as in theolfactory bulb, oligodendrocytes are also depleted, and myelinationis reduced in proportion to the reduced mitral mass. These datamake a strong case for the primacy of axonal factors other thanIGF1 in determining oligodendrocyte survival and myelination.

  FOOTNOTES

Received Feb. 27, 1998; revised April 24, 1998; accepted May 6, 1998.

Correspondence should be addressed to Dr. Clara Cheng, Building 10/10N262, 10 Center Drive, National Institutes of Health,Bethesda, MD 20892.

  REFERENCES

Top
Abstract
Introduction
Materials & Methods
Results
Discussion
References

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