Peripheral Infusion of IGF-I Selectively Induces Neurogenesis in the Adult Rat Hippocampus

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The Journal of Neuroscience, April 15, 2000, 20(8):2896-2903

Peripheral Infusion of IGF-I Selectively Induces Neurogenesis in the Adult Rat Hippocampus
Maria A. I. Åberg¹, N. David Åberg¹, Helena Hedbäcker¹, Jan Oscarsson², and Peter S. Eriksson¹
¹ Institute of Clinical Neuroscience, Sahlgrenska University Hospital, and ² Department of Physiology and Pharmacology, Göteborg University, Göteborg, Sweden

  ABSTRACT

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

In several species, including humans, the dentate granule cell layer (GCL) of the hippocampus exhibits neurogenesis throughoutadult life. The ability to regulate adult neurogenesis pharmacologicallymay be of therapeutic value as a mechanism for replacing lostneurons. Insulin-like growth factor-I (IGF-I) is a growth-promotingpeptide hormone that has been shown to have neurotrophic properties.The relationship between IGF-I and adult hippocampal neurogenesisis to date unknown. The aim of this study was to investigate theeffect of the peripheral administration of IGF-I on cellular proliferationin the dentate subgranular proliferative zone, which containsneuronal progenitor cells, and on the subsequent migration anddifferentiation of progenitor cells within the GCL. Using bromodeoxyuridine(BrdU) labeling, we found a significant increase of BrdU-immunoreactiveprogenitors in the GCL after 6 d of peripheral IGF-I administration.To determine the cell fate in progenitor progeny, we characterizedthe colocalization of BrdU-immunolabeled cells with cell-specificmarkers. In animals treated with IGF-I for 20 d, BrdU-positivecells increased significantly. Furthermore, the fraction of newlygenerated neurons in the GCL increased, as evaluated by the neuronalmarkers Calbindin D_28K, microtubule-associated protein-2, andNeuN. There was no difference in the fraction of newly generatedastrocytes. Thus, our results show that peripheral infusion ofIGF-I increases progenitor cell proliferation and selectivelyinduces neurogenesis in the progeny of adult neural progenitorcells. This corresponds to a 78 ± 17% (p < 0.001) increase inthe number of new neurons in IGF-I-treated animals compared withcontrols.

Key words: brain; rat; IGF-I; insulin-like growth factor-I; stem cell; progenitor cell; hippocampus; neurogenesis; stereology

  INTRODUCTION

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Most CNS neurons are terminally differentiated and are, thus, not replaced after neuronal cell death. However, self-renewingcells with multilineage potential, designated stem cells or progenitorcells, have been identified in the adult mammalian brain (Reynoldsand Weiss, 1992; Richards et al., 1992; Craig et al., 1996; Suhonenet al., 1996; McKay, 1997; Temple and Alvarez-Buylla, 1999). Neuralstem cells generate new neurons throughout life in the dentategyrus of the hippocampus in several species, including humans(Altman and Das, 1965; Kuhn et al., 1996; Eriksson et al., 1998).Progenitor cells isolated from this region have demonstrated thecapacity for self-renewal in vitro; when grafted back into theadult brain, they have the potential to develop into mature neuronswith the phenotypic characteristics of surrounding neurons (Suhonenet al., 1996). Proliferation and differentiation of adult neuralstem cells are affected by age, growth factors, excitatory input,adrenal steroids, seizures, and enrichment of the environment(Cameron and Gould, 1994; Palmer et al., 1995; Craig et al., 1996;Kuhn et al., 1996; Bengzon et al., 1997; Gould et al., 1997; Kempermannet al., 1997; McKay, 1997; Nilsson et al., 1999). However, thereare to our knowledge no known exogenous substances that selectivelyinduce neurogenesis in the adult mammalian CNS in vivo.

Insulin-like growth factor-I (IGF-I) is a growth-promoting peptide that is important during development of the brain (Saraand Carlsson-Skwirut, 1988; Bozyczko-Coyne et al., 1993; Giacobiniet al., 1995; Dentremont et al., 1999). Overexpression of IGF-I,both peripherally and centrally, in transgenic mice results inan increase in brain size and myelin content (Carson et al., 1993).Conversely, the number of granule cells in the hippocampus, theoligodendrocyte and neuron density within the olfactory bulbs,and total brain size are reduced in knock-out mice (Beck et al.,1995; Cheng et al., 1998).

There are two potential pathways by which IGF-I may affect the hippocampus. IGF-I receptors expressed in the adult dentategyrus (Lesniak et al., 1988) may be reached by IGF-I either fromthe periphery (by crossing the blood-brain barrier) (Duffy etal., 1988; Reinhardt and Bondy, 1994) or locally by paracrineIGF-I (Breese et al., 1996). In the present study we wanted toassess the impact of peripheral, normally liver-derived, IGF-I.

It is possible that the reported alterations in hippocampal granule cell number in animals with supranormal or subnormal IGF-Ilevels occur in part as a result of a perturbation in the proliferationof endogenous neural progenitor cells. This hypothesis led usto investigate the proliferation and differentiation of progenitorcells in the adult dentate gyrus in hypophysectomized (hx) ratstreated with peripheral administration of IGF-I. The hx rat iswidely used as a model of somatic IGF-I deficiency because hxanimals have low circulating levels of IGF-I (Schoenle et al.,1982; Sjöberg et al., 1994). We used bromodeoxyuridine (BrdU)labeling to monitor proliferation and double or triple immunofluorescentlabeling for BrdU and cell-specific markers to determine the phenotypeof the progenitorprogeny.

  MATERIALS AND METHODS

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ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Animals and hormonal treatment. We used hx rats, which have low circulating levels of IGF-I (Schoenle et al., 1982; Sjöberget al., 1994). The effect of IGF-I treatment was shown by comparingthe weight gain in treated versus untreated (control) hx rats(data not shown) (Schoenle et al., 1982; Fielder et al., 1996).Female Sprague Dawley rats (Møllegaard Breeding Center, Ejby,Denmark) were hypophysectomized at 50 d of age at the MøllegaardBreeding Center. Weight-matched female normal (non-hx) rats werealso investigated. All rats were maintained under standard conditionsof temperature (24-26°C) and humidity (50-60%) and with lightson between 05:00 and 19:00 hr. The rats had access to water andstandard laboratory chow ad libitum. Hormonal treatment started7-10 d after hypophysectomy. All hx rats received subcutaneousinjections of cortisol phosphate (400 µg/kg per d; Solu-Cortef,Upjohn, Puurs, Belgium) and L-thyroxine (10 µg/kg per d; NycomedPharma, Oslo, Norway) diluted in saline (08:00 hr) (Sjöberg etal., 1994). L-Thyroxine and glucocorticoids were given becausethese hormones are known to be important for normal central neuralplasticity and function (Sinha et al., 1994; McEwen, 1996; Reaganand McEwen, 1997). Control hx rats were given cortisol and L-thyroxine.Recombinant human IGF-I (Genentech, South San Francisco, CA) wasdiluted in saline and given as a continuous infusion using Alzet2001 osmotic minipumps (Alza, Palo Alto, CA; 1.25 mg/kg per d)for short-term experiments and Alzet 2004 (0.9 mg/kg per d) forlong-term experiments, resulting in comparable levels of serumIGF-I (see Results). The osmotic minipumps were implanted subcutaneouslyon the backs of the rats. Hormonal treatment continued for 6 d(short-term) or 20 d (long-term). Altogether three separate setsof animals were used (one short-term and two long-term). Duringthe first 5 d of each treatment period, all animals received adaily intraperitoneal injection of bromodeoxyuridine (BrdU; 50mg/kg of body weight; Boehringer Mannheim, Scandinavia AB, Bromma,Sweden). The animals were killed by decapitation at the end ofeach treatment period. The experimental methods were approvedby the Board of Animal Ethics (Göteborg University, Göteborg,Sweden).

Immunohistochemistry. After decapitation, the brains were removed and fixed in 4% p-formaldehyde for 24 hr and stored thereafterin a 30% sucrose solution. Coronal sections (40 µm) obtained bythe use of a freezing microtome were stored in a cryoprotectant(25% ethylene glycol and 25% glycerin in a 0.05 M phosphate buffer)at $-$ 20°C before immunohistochemistry or immunofluorescence. Stainingwas done on free-floating 40 µm sections pretreated with 0.6%H₂O₂ in Tris-buffered saline (TBS; 0.15 M NaCl and 0.1 M Tris-HCl,pH 7.5) for 30 min to block endogenous peroxidase activity. Toensure the detection of BrdU-labeled nuclei, we denatured theDNA before incubation with mouse anti-BrdU antibody (1:400; BoehringerMannheim). DNA denaturation was performed in the following manner:tissue was incubated in 50% formamide and 2× SSC (1× SSC, 0.3M NaCl and 0.03 M sodium citrate) for 2 hr at 65°C, rinsed for15 min in 2× SSC, incubated again for 30 min in 2 M HCl at 37°C,and rinsed again for 10 min in 0.1 M boric acid at pH 8.5. Thetissue was then rinsed in TBS several times, followed by incubationin TBS, 0.25% Triton X-100, and 3% normal horse serum (TBS-TS)for 30 min and then with primary antibody in TBS-TS overnightat 4°C. The tissue sections were then incubated for 2 hr withbiotinylated horse anti-mouse IgG (1:160) secondary antibodies(Vector Laboratories, Burlingame, CA) and rinsed in TBS. Avidin $---$ biotin-peroxidasecomplex was applied for 1 hr before 5 min of peroxidase detection(using 0.25 mg/ml diaminobenzidine, 0.01% H₂O₂, and 0.04%NiCl).

Immunofluorescence. Sections were treated for DNA denaturation, as described above, and then incubated in TBS-TS for 30 min.Thereafter, they were incubated with rabbit anti-Calbindin D_28K(1:500; SWant, Bellinzona, Switzerland), mouse NeuN (1:30; Chemicon,Temecula, CA), mouse microtubule-associated protein-2 (MAP2; 1:400;Boehringer Mannheim, Mannheim, Germany), or rabbit anti-GFAP (1:500;Dako, Glostrup, Denmark) and rat anti-BrdU antibody (1:200; Harlan,Loughborough, United Kingdom) overnight at 4°C. GFAP and CalbindinD_28K were detected with Texas Red-conjugated anti-rabbit IgG (1:200for GFAP and 1:100 for Calbindin D_28K; Jackson ImmunoResearch,West Grove, PA), Calbindin D_28K was also detected with Cy5-conjugatedanti-rabbit IgG (1:150; Jackson ImmunoResearch), NeuN and MAP2were detected with Texas Red-conjugated anti-mouse IgG (1:100;Jackson ImmunoResearch), and BrdU was labeled with an FITC-conjugatedanti-rat IgG (1:150; Jackson ImmunoResearch) for 2 hr at 37°C.Immunofluorescence was detected and processed with a Nikon Diaphotfluorescence microscope and confocal laser-scanning microscopyusing a Bio-Rad 1024 system (Hercules,CA).

Quantification. For each animal, the number of BrdU-positive cells in the granule cell layer (GCL; including the subgranularlayer) and in the hilus and their corresponding sample volumeswere determined in 12 immunoperoxidase-stained, 40-µm-thick coronalsections taken 240 µm apart. Area estimations were obtained byplanimetry, using a Lucivid device (MicroBrightField, Colchester,VT) attached to a Leica microscope. The section thickness of 40µm (microtome setting) was used in the dissector estimation ofvolume. The number of BrdU-positive cells was counted within theGCL and two cell diameters below the GCL, ignoring the cells inthe uppermost focal plane and focusing through the thickness ofthe section to avoid errors caused by oversampling [for a discussionof the optical dissector principle, see Gundersen et al. (1988);West (1993); Coggeshall and Lekan (1996)]. Pictures were takenunder a Nikon microscope equipped with a video camera. The resultsare expressed as BrdU-positive cells per sample volume per section.We determined the total number of BrdU-positive cells in the GCLand in the hilus. We also determined the colocalization of BrdUwith cell-specific markers in the GCL in six to eight 40-µm-thickcoronal sections taken 240 µm apart in each animal. For the neuronalmarker Calbindin D_28K, 457 BrdU-positive cells were analyzed respectingcolocalization; for the neuronal marker NeuN, 735 BrdU-positivecells were analyzed; for the neuronal marker MAP2, 203 BrdU-positivecells were studied; and for the glial marker GFAP, 911 BrdU-positivecells were analyzed. All cell-counting procedures were blindlyperformed. The absolute volumes of the GCL and the hilus weredetermined in a Nissl-stained series of sections taken 480 µmapart throughout thehippocampus.

IGF-I measurement. Serum IGF-I concentrations were determined by a hydrochloric acid-ethanol extraction RIA, using human IGF-Ifor labeling (Nichols Institute Diagnostics, San Juan Capistrano,CA) (Sjöberg et al., 1994).

Statistical analysis. Values are expressed as the mean ± SEM. Comparisons between groups were made with one-way ANOVA throughoutthe study. Two-way ANOVA was applied to the results on colocalizationof BrdU and Calbindin D_28K/NeuN. Regression analysis with correlationanalysis was also performed. Differences that are not statisticallysignificant are followed by the abbreviation NS. p values < 0.05were considered statisticallysignificant.

  RESULTS

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

IGF-I stimulates proliferation of neural progenitors in the adult rat dentate gyrus

Two IGF-I treatment protocols were used in the IGF-I-deficient hypophysectomized rats. The 6 d treatment was performed toevaluate the short-term effect of IGF-I on proliferation, andthe 20 d treatment was used to evaluate effects on the cell fateof BrdU-immunoreactive progenitorprogeny.

Blood samples were taken when the animals were killed; serum levels of IGF-I were measured to make sure that the miniosmoticdelivery system was functioning properly. One day after the lastinjection of BrdU in animals treated for 6 d, the serum levelwas 148 ± 35 µg/dm³ compared with 47 ± 1.6 µg/dm³ in hx controls (p < 0.01). Fifteen days after the last injectionof BrdU in animals treated for 20 d, the serum level was 222 ±23 µg/dm³ in IGF-I-treated animals compared with 65 ± 7.0 µg/dm³ in hx controls (p < 0.001). Additionally, the weight gain ofrats treated with IGF-I showed the expected response (data notshown). Together, these data show that the peripheral infusionof IGF-I reached the systemic circulation, thereby being ableto affect the brain by passing the blood-brainbarrier.

The number of newly generated cells in the adult dentate gyrus was determined by monitoring the incorporation and subsequentimmunohistochemical detection of BrdU within the nuclei of dividingcells (Fig. 1b-e). BrdU-immunoreactive nuclei were located predominantlywithin the GCL or along the border between the GCL and the hilus.The nuclei were generally condensed and exhibited variable shapes.The number of BrdU-immunoreactive cells in IGF-I-treated animalswas compared with the number of BrdU-immunoreactive cells in thehx controls. In animals that underwent short-term (6 d) IGF-Itreatment [i.e., animals evaluated 1 d post-BrdU injection (p.i.)],the number of BrdU-immunoreactive cells in the GCL was 7291 ±950 cells/mm³ compared with 4076 ± 731 cells/mm³ in hx controls, which corresponds to a 79 ± 29% increase (p =0.015) (Fig. 2a). In the hilus, the number of BrdU-immunoreactivecells was 2765 ± 331 cells/mm³ in IGF-I-treated animals compared with 1808 ± 211 cells/mm³ in hx controls (p < 0.05).

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Figure 1. BrdU immunohistochemistry in two experiments in which IGF-I was given for 6 d (corresponding to 1 d p.i. of BrdU) or 20 d (corresponding to 15 d p.i. of BrdU). a, The hippocampal region of the adult rat brain immunoperoxidase-stained for the neuronal marker Calbindin D_28K. b-e, Differential interference contrast photomicrographs of BrdU-immunopositive cells in the hippocampus. A comparison of BrdU labeling in controls (b, d) and IGF-I-treated animals (c, e) at 1 and 15 d p.i. of BrdU is shown. (For quantification, see Fig. 2.) Scale bar, 100 µm.

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Figure 2. Quantification of BrdU-positive cells in the adult rat hippocampus. A, The density of BrdU-positive cells (cells per cubic millimeter of sample volume) in the GCL 1 and 15 d p.i. was determined stereologically. IGF-I-treated animals (n = 4 at 1 d p.i.; n = 7 at 15 d p.i.) are hx rats given L-thyroxine, cortisol, and IGF-I, as described in Materials and Methods. Controls (n = 5 at 1 d p.i.; n = 8 at 15 d p.i.) are hx rats given L-thyroxine and cortisol only. Means ± SEM are given. *p < 0.05; **p < 0.01. B, Weight gain and the number of BrdU-labeled cells in the GCL at the individual level are compared. There is a correlation between S-IGF-I and BrdU-positive cells after 20 d of IGF-I treatment (15 d p.i.); animals with a relatively low serum IGF-I have relatively low numbers of BrdU-positive cells, and vice versa.

In animals that underwent long-term (20 d) IGF-I treatment (i.e., those evaluated 15 d p.i.), the number of BrdU-immunoreactivecells in the GCL was 2695 ± 175 cells/mm³ in IGF-I-treated animals compared with 1883 ± 138 cells/mm³ in hx controls, which corresponds to a 43 ± 12% increase (p <0.01) (Fig. 2 A). In the hilus, the number of BrdU-immunoreactivecells was 640 ± 56 cells/mm³ in IGF-I-treated animals compared with 306 ± 62 cells/mm³ in hx controls (p < 0.01).

In normal (nonhx) rats, the number of BrdU-immunoreactive cells detected 15 d p.i. was 2416 ± 283 cells/mm³ in the GCL (n = 8), which is close to that in the IGF-I-treatedhx rats. This observation supports a role for IGF-I in the regulationof neurogenesis in the GCL. Furthermore, a statistically significantpositive correlation between weight gain and the number of BrdU-positivecells in the GCL was observed (r = 0.92; p < 0.01) (Fig. 2 B).This observation demonstrates that a stronger biological activityof IGF-I in the periphery also has a greater effect on hippocampalneurogenesis.

The absolute volume of the GCL and of the hilus and the ratio between these volumes were determined in animals that underwentlong-term IGF-I treatment. There were no significant differencesin the volume of the GCL and of the hilus or between the ratiosof these volumes in IGF-I-treated animals versus animals in thehx control group (data notshown).

IGF-I selectively induces neurogenesis

Colocalization of BrdU immunoreactivity with immunoreactivity of the granule cell marker Calbindin D_28K (Fig. 3a-h) and theastrocyte marker GFAP (Fig. 3i) was investigated to determinethe phenotype of progenitor cell progeny in the dentate gyrusafter long-term IGF-I therapy (i.e., in animals evaluated 15 dp.i.) compared with that of hx controls. Using confocal microscopy,we were able to detect colocalization of BrdU with either CalbindinD_28K or GFAP in the GCL. In IGF-I-treated hx animals, we foundan increase in the Calbindin D_28K- and BrdU-immunoreactive cellfraction (from 43 ± 1.5 to 54 ± 3.0%) compared with that of hxcontrols; this corresponds to a 26 ± 9% (p < 0.01) increase (Fig.4). In addition, 17 ± 1.1% of BrdU-positive cells were also GFAPpositive compared with 20 ± 1.3% in hx controls (NS). In the hilus,no colocalization of BrdU and Calbindin D_28K was found in IGF-I-treatedor control animals, whereas BrdU colabeled with GFAP in 27 ± 1.4%of BrdU-positive cells in IGF-I-treated animals compared with23 ± 2.5% in controls (NS). To confirm that the increase of BrdU-andCalbindin D_28K-immunolabeled cells represented new neurons, weperformed additional double- and triple-immunolabeling characterizationswith other neuronal markers, namely, MAP2 and NeuN. We found thatall (100%) of the newly generated BrdU- and Calbindin D_28K-positiveneurons are MAP2 positive. We also found an increase in the fractionof BrdU- and NeuN-labeled cells (from 54 ± 5.0 to 65 ± 4.0%) inIGF-I-treated animals compared with controls. A two-way ANOVAof these data, using treatment and type of antibodies as factors,shows that IGF-I treatment results in an increase in the fractionof newly generated neurons (p < 0.01). Together, these data showthat long-term treatment with IGF-I affected differentiation intoneurons but not into astrocytes.

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Figure 3. Colocalization of BrdU immunoreactivity (green-yellow in a, c-i, l, m, o, p) with immunoreactivity of the granule cell marker Calbindin D_28K (red in a-h; blue in j, m), the astrocyte marker GFAP (red in i), the neuronal marker MAP2 (red in k, m), or the neuronal marker NeuN (red in n, p) (arrows indicate colocalization in a-p). Red blood cells and endothelial cells in several small blood vessels also emit nonspecific green and red fluorescence (asterisks in a-p). The specificity of BrdU and Calbindin D_28K coexpression in three dimensions is demonstrated by a Z-series of focal planes above (e, f) and below (g, h) the focal plane shown in d (arrows in e-h indicate the same cell as in d). The merged image of b and c is shown in d, the merged image of j, k, and l is shown in m, and the merged image of n and o is shown in p. Insets of each boxed area in j-m are magnified 2.5×. Scale bars: a, i, 50 µm; b $---$ h, j $---$ m, n $---$ p, 25 µm.

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Figure 4. Percentage of the surviving BrdU-positive cells after 20 d of IGF-I treatment that differentiated into either neurons or astrocytes. Colocalization of BrdU immunoreactivity with cell-specific markers, either the granule cell marker Calbindin D_28K or the astrocyte marker GFAP, was monitored to determine the phenotype of newborn cells after treatment with IGF-I, when compared with controls in the GCL (n = 5 for controls; n = 7 for IGF-I-treated animals). Means ± SEM are given. **p < 0.01.

To determine the total number of newly generated neurons, we determined the absolute volume of the GCL (data not shown) andmultiplied this by the number of cells per sample volume after20 d of IGF-I treatment (Fig. 2 A) and the ratio of CalbindinD_28K-/BrdU-positive cells (Fig. 4) for each respective group.We found that there were a total of 1971 ± 154 newly generatedneurons in IGF-I-treated hx animals compared with 1106 ± 107 inhx controls. This corresponds to a 78 ± 17% (p < 0.001) increasein the number of newly generated neurons in IGF-I-treatedanimals.

  DISCUSSION

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

We investigated the effects of IGF-I on the proliferation and differentiation of neural progenitor cells in the adult rathippocampus. A substantial increase in the total number of BrdU-immunoreactivecells was observed after 6 d of IGF-I administration, demonstratingthe proliferative effect of IGF-I. Furthermore, an analysis ofthe phenotypic distribution after 20 d of IGF-I treatment indicatedthat the number of newly generated neurons in the GCL increasedsignificantly. To our knowledge, this is the first study showinga selective induction of neurogenesis in the adult mammalianCNS.

It has been demonstrated that the incorporation of BrdU into hippocampal granule cells reflects the number of proliferatingprogenitor cells. The thymidine analog BrdU is incorporated intoDNA and can be detected immunohistochemically in cell progeny(del Rio and Soriano, 1989; Kuhn et al., 1996). Bioavailabilityof BrdU after injection has been estimated to last ~2 hr, andBrdU labels DNA only during the S phase, which has been estimatedto last ~8 hr (Nowakowski et al., 1989; Takahashi et al., 1992).Thus, the regimen used in this study is not likely to cause anoverestimation of the number of proliferating cells, because oneinjection cannot label all dividing cells during a 24 hr period.The resulting BrdU-positive cells also include the progeny oflabeled cells that divided again after BrdU was discontinued.Although these cells still represent newborn cells, the exacttime of cell division is unknown; therefore, injections of BrdUover a 5 d period should reduce the proportion of BrdU-positivecells that divide again compared with a single dose of BrdU. The5 d treatment period should also reduce the significance of anytreatment-induced alterations in the length of any phase of thecellcycle.

Peripheral-derived IGF-I stimulates neurogenesis in the dentate gyrus

The main regulators of circulating levels of IGF-I are nutritional factors and growth hormone (GH) (Humbel, 1990; Thissenet al., 1994). IGF-I is expressed in most tissues in the body,including large organs like skeletal muscle (Isgaard et al., 1988),adipose tissue (Vikman et al., 1991), and liver (Schwander etal., 1983; D'Ercole et al., 1984; Humbel, 1990). However, theliver-derived IGF-I is the principal source of circulating IGF-Ithat is able to affect the brain (Schwander et al., 1983; Sjögrenet al., 1999).

The administration of IGF-I results in weight gain in hypophysectomized animals, and this fact has been used in previous studiesto verify the bioactivity of exogenous IGF-I (Schoenle et al.,1982; Fielder et al., 1996). The data showing a correlation betweenweight gain and the proliferation rate of neural progenitors arenoteworthy, because they support the existence of a relationshipbetween the effect of IGF-I on peripheral tissue and that on theCNS and thus suggest that circulating IGF-I isneurotrophic.

Possible mechanisms of IGF-I-induced neurogenesis in the adult dentate gyrus

We show that peripheral administration of IGF-I induces neurogenesis in the adult hippocampus. In our study, the number ofnewly generated neurons represents a combination of the proliferativerate, the differentiation rate, and net cell survival/apoptosis.This assumption is supported by other studies, in which IGF-Iincreased the proliferation of embryonic CNS precursors in vitro(DiCicco-Bloom and Black, 1988; Drago et al., 1991; Zackenfelset al., 1995) and in vivo (Ye et al., 1996), and conversely, thenumber of hippocampal granule neurons was reduced in studies ofIGF-I knock-out mice (Beck et al., 1995). These results are consistentwith our data on the adult rat, which demonstrate a pronouncedincrease in the number of BrdU-positive cells after 6 d of IGF-Itreatment and suggest that a considerable proportion of the newbornneurons detected after 20 d of IGF-I treatment is attributableto stimulation of progenitor cellproliferation.

We further show that differentiation is also affected by IGF-I, because an increase was seen not only in the absolute numberof cells but also in the fraction of newly generated neurons.Similarly, IGF-I stimulates mouse embryonic CNS neural precursorsto differentiate into non-GABAergic neurons in vitro (Arsenijevicand Weiss, 1998). In vivo, IGF-I increases neuronal recruitmentfrom the adult songbird subependymal zone (Jiang et al., 1998).Together, our observations and the observations of others supportthe hypothesis that IGF-I increases neuronal differentiation inboth the developing and adult CNS. However, a third possibility $---$ aneffect on cell survival/apoptosis $---$ could also be responsible forthe increase in neurons observed after IGF-I treatment, becauseIGF-I supports the survival of neurons in the embryo (Bozyczko-Coyneet al., 1993; Hughes et al., 1993; Lindholm et al., 1996; Blairet al., 1999). The knowledge is still limited about the role ofapoptosis in the regulation of adult neurogenesis. Because apoptoticnuclei have been described in the subgranular zone, cell eliminationby programmed cell death could explain the decrease in BrdU-positivecells observed 15 d p.i. compared with 1 d p.i. (Bengzon et al.,1997). Quantitatively, the loss of BrdU-positive cells might reflectan overestimation of apoptosis, because BrdU itself could damagesome labeled cells. The fact that IGF-I has been shown to attenuateapoptosis in hippocampal neurons after ischemia (Tagami et al.,1997) suggests that the observed increase in the fraction of newbornneurons after IGF-I treatment is in part an effect on cellsurvival.

Potential of induced neurogenesis in the dentate gyrus

It has been suggested that an increase in the expression of the IGF-I gene or peripherally administered IGF-I plays an importantrole in the neurotrophic response after injury such as epilepsyor ischemia in the adult rat brain (Gluckman et al., 1992; Guanet al., 1993; Breese et al., 1996; Saatman et al., 1997; Tagamiet al., 1997; Liu et al., 1998; Hughes et al., 1999). Severaldisorders are associated with GCL pathology. Epilepsy is associatedwith granule cell pathophysiology, including changes in hippocampalcalbindin immunoreactivity in rats (Köhr et al., 1991). Similarly,temporal lobe seizures and memory dysfunction are associated withabnormalities in the GCL and hilus (Lowenstein et al., 1992; Beachet al., 1995).

Also, ischemic injury causes neuronal cell loss in the hippocampus and subsequent memory impairment in animals and humans(Zola Morgan et al., 1992; Squire and Zola, 1996). Consideringthat dentate neurogenesis is increased with enriched environmentand learning (Kempermann et al., 1997, 1998; Gould et al., 1999;Nilsson et al., 1999), it is plausible that new neurons actuallyparticipate in and mediate this process. The opposite order ofevents is also very exciting and may also hold true, i.e., improvedability of memory formation after for example drug-induced neurogenesis.This however is a very complex process and remains to be proven.The relationship between memory and adult neurogenesis is supportedfurther by the fact that radiation, which is known to impair memory(Leibel and Sheline, 1987), also inhibits GCL neurogenesis (Parentet al., 1999). Probably IGF-I-stimulated proliferation and neurogenesisin neural progenitors play a role in reducing neuronal loss afterhippocampal damage as occurs with epilepsy and ischemia. Thisissue, however, warrants furtherinvestigation.

In conclusion, our in vivo data of selective induction of neurogenesis by peripheral IGF-I on hippocampal progenitors suggesta role for this substance in the generation of new neurons inthe adult hippocampus. Additional studies of the effects of IGF-Imay therefore yield novel ideas with possible implications forfuture therapeuticapproaches.

  FOOTNOTES

Received Oct. 21, 1999; revised Feb. 7, 2000; accepted Feb. 7, 2000.

This study was supported by grants from the Swedish Medical Research Council (project no. 12X-12535), the Faculty of Medicineof the University of Göteborg, the John and Brit WennerströmsFoundation for Neurological Research, the Rune and Ulla AmlövsFoundation for Neurological and Rheumatological Research, StiftelsenGöteborgs MS förenings forsknings och byggnadsfond, StiftelsenHandlanden Hjalmar Svenssons Forskningsfond, the Swedish Societyof Medicine, Göteborgs Läkaresällskap, the Edit JacobssonsFoundation, Stiftelsen Thure Carlssons Minne, Stiftelsen LarsHiertas Minne, the Novo Nordisk Foundation, the Åke Wiberg Foundation,the Magnus Bergvalls Foundation, Axel Linders stiftelse, and theTore Nilssons Foundation. We appreciate the technical advice ofAnn-Marie Alborn and the assistance of Barbro Eriksson with codingslides. We also want to thank Maria Wågberg and Knut Petterssonat Astra Hässle Gothenburg for kindly letting us use their microscope.Recombinant human IGF-I was a kind gift from Genentech (SouthSan Francisco, CA). We are grateful to Dr. Tommy Johnson at theDepartment of Statistics (Göteborg University, Göteborg, Sweden)for the statistical advice and to Proper English (Alfta, Sweden)for proofreading of this manuscript inEnglish.
Correspondence should be addressed to Dr. Peter S. Eriksson, Institute of Clinical Neuroscience, Göteborg University, BlåStråket 7, SE-413 45 Göteborg, Sweden. E-mail: per{at}neuro.gu.se.

  REFERENCES

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
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