Insulin-Like Growth Factor-I Overexpression Attenuates Cerebellar Apoptosis by Altering the Expression of Bcl Family Proteins in a Developmentally Specific Manner

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The Journal of Neuroscience, March 1, 2001, 21(5):1481-1489

Insulin-Like Growth Factor-I Overexpression Attenuates Cerebellar Apoptosis by Altering the Expression of Bcl Family Proteins in a Developmentally Specific Manner
Dionisios Chrysis, Ali Suha Calikoglu, Ping Ye, and A. Joseph D'Ercole
Department of Pediatrics, The University of North Carolina, Chapel Hill, North Carolina 27599-7220

  ABSTRACT

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

In studies of transgenic (Tg) mice that overexpress insulin-like growth factor-I (IGF-I) exclusively in the CNS, we demonstrateda dramatic increase in cerebellar granule cell number that appearedto be attributable predominantly to enhanced survival. IGF-I anti-apoptoticactions are well established in cultured neurons, but comparablestudies in vivo are few. Using the same Tg mice, therefore, weset out to document IGF-I anti-apoptotic effects during cerebellardevelopment and to probe IGF-I signaling mechanisms. Comparedwith cerebella (CBs) of non-Tg littermates, those of Tg mice hadfewer apoptotic cells at postnatal day 7 (P7) and showed a similartendency at P14 and P21. At each age studied, procaspase-3 andcaspase-3 were decreased in CBs of Tg mice. The caspase-3 declinewas accompanied by decreases in the 85 kDa fragment of Poly(ADP-ribose)polymerase, a known product of caspase cleavage, suggesting decreasedcaspase activity. At P7 decreased apoptosis in Tg mice was associatedwith increased expression of the anti-apoptotic Bcl genes, Bcl-x_Land Bcl-2. The mRNA expression of the proapoptotic Bcl genes,Bax and Bad, also was increased, but no changes were observedin the abundance of their proteins. At P14 Bcl-xL and Bcl-2 expressionwere similar in normal and Tg mice; Bax mRNA was unchanged inTg mice, but its protein abundance was decreased, and both BadmRNA and protein abundance were decreased. At P21 Bcl-xL and Bcl-2expression were unchanged, but Bax and Bad expression were decreased.Our data show that IGF-I exerts anti-apoptotic actions duringcerebellar development, and thereby alters the magnitude of naturallyoccurring apoptosis. IGF-I appears to affect multiple steps inthe apoptotic pathway in a developmentally specific manner. IGF-Idecreases caspase-3 availability and activity, increases the expressionof anti-apoptotic Bcl-x_L and Bcl-2 during early postnatal development,and decreases proapoptotic Bax and Bad expression at later developmentalstages.

Key words: IGF-I; apoptosis; cerebellum; development; transgenic mice; Bcl; Bcl-2; Bcl-x_L; Bad; Bax; caspase-3; Poly(ADP-ribose) polymerase

  INTRODUCTION

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ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Insulin-like growth factor-I (IGF-I) plays a significant role in the stimulation of brain development (D'Ercole et al., 1996).IGF-I overexpression in the brains of transgenic (Tg) mice resultsin brain overgrowth (Carson et al., 1993; Ye et al., 1995, 1996)that is characterized by an increase in neuron and oligodendrocytenumber and a marked increase in myelination. The increase in cellnumber in IGF-I Tg mice appears to be attributable to both stimulationof proliferation and an inhibition of apoptosis. Mice with targeteddisruptions of both IGF-I alleles have small brains with decreasedmyelination and a reduction or absence in certain neuron populations(Baker et al., 1993; Liu et al., 1993), and mice that lack expressionof the type I IGF receptor have a similar phenotype (Baker etal., 1993; Liu et al., 1993). Many studies of cultured cells (Matthewsand Feldman, 1996; Baserga et al., 1997), including those of culturedneurons and oligodendrocytes (Baker et al., 1999; Ye and D'Ercole,1999), demonstrate that IGF-I is capable of promoting cell survival.Investigations into whether IGF-I acts in vivo to inhibit apoptosis,however, arefew.

In studies of one of our lines of IGF-I Tg mice, we obtained evidence indicating that IGF-I stimulates cerebellar overgrowthprimarily by inhibiting apoptosis (Ye et al., 1996). These micecarry a fusion gene that uses the mouse 5' genomic regulatoryregion of the IGF-II gene to drive a human IGF-I cDNA (IGF-II/IGF-ITg mice). This transgene is expressed throughout the brain beginningabout the time of birth and exhibits highest expression in cerebellum(CB). Compared with normal littermates, the brains of heterozygousIGF-II/IGF-I Tg mice exhibit overgrowth from the second week ofpostnatal life with the CB exhibiting the greatest increase insize, such that by postnatal day 50 (P50) cerebellar weight isincreased by 90%. The increased weight is attributable to an increasein the total number of granule and Purkinje cells (82 and 20%increases, respectively). Granule cell proliferation is modestlyincreased only at P15, making it unlikely that it is sufficientto account for the nearly twofold increase in granule cell number.Increased cell survival, therefore, appears to account for theincreased cerebellar granule cell number. Several other studiesof intact mice provide evidence consistent with IGF-I anti-apoptoticactions on neurons: (1) IGF-I gene expression is low in the Purkinjecell degeneration (pcd) mice, a mutant mouse line characterizedby increased cerebellar apoptosis (Zhang et al., 1997), and (2)IGF-I treatment before experimental cerebral ischemia attenuatesapoptosis in hippocampal neurons (Tagami et al., 1997).

The mechanisms by which IGF-I prevents cultured cells from entering a death program have not been defined, and both the phosphatidylinositol3'-kinase (PI3-K) and the mitogen-activated protein kinase (MAP-K)pathways (Kulik et al., 1997; Parrizas et al., 1997) have beenimplicated. Furthermore, a number of in vitro studies link IGF-Iactions to the Bcl family of proteins, but these findings aresomewhat discrepant. For example, IGF-I inhibition of apoptosisis associated with: (1) increased Bcl-x_L expression and action(Singleton et al., 1996; Parrizas and LeRoith, 1997); (2) increasedBcl-2 expression (Minshall et al., 1997); (3) suppressed interleukin-1 $beta$ -convertingenzyme (caspase)-mediated cell death, apparently through a mechanismindependent of the expression of Bcl-2, Bcl-x_L, and Bax (Junget al., 1996), and (4) an inactivation of Bad by phosphorylation(del Peso et al., 1997; Dudek et al., 1997). It seems likely thatIGF-I anti-apoptotic actions differ among cell types, at leastwhen studied in culture. Studies of IGF-I anti-apoptotic effectsin vivo are essential, therefore, to clarify the mechanisms bywhich IGF-I influencesapoptosis.

Apoptosis leads to a massive loss of granule cells during active neurogenesis in the first three postnatal weeks of cerebellardevelopment (Landis and Sidman, 1978; Wood et al., 1993). BecauseIGF-I overexpression in IGF-II/IGF-I Tg mice occurs when cerebellarapoptosis is active, study of these Tg mice is especially usefulto probe IGF-I anti-apoptotic effects. We hypothesized that cerebellarovergrowth in these Tg mice is attributable, at least in largepart, to IGF-I inhibition of granule cell apoptosis and that theseIGF-I actions are regulated by alterations in the expression ofgenes for the Bcl family ofproteins.

  MATERIALS AND METHODS

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ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Reagents. PCR reagents, DNA polymerase, digoxigenin and biotin-labeled nucleotides, digoxigenin chemiluminescent detectionreagents, and positively charged nylon membranes were purchasedfrom Roche Molecular Biochemicals (Indianapolis, IN). Reversetranscriptase, RNA polymerase and restriction enzymes were purchasedfrom Promega (Madison, WI), and a purification system for PCRproducts was purchased from Qiagen (Chatsworth, CA). Reagentsfor RNase protection assay (RPA) and detection system were obtainedfrom Ambion (Austin, TX). Trizol for RNA extraction was purchasedfrom Life Technologies (Grand Island, NY). Polyvinylidene difluoride(PVDF) membranes, protein molecular standards, and ECL ^plus chemiluminescent system for Western immunoblots were from Amersham(Arlington Heights, IL), rabbit polyclonal antibodies againstBcl-x, Bax, Bad, Poly(ADP-ribose) polymerase (PARP), and caspase-3were from Santa Cruz Biotechnology (Santa Cruz, CA), and Bcl-2was from Upstate Biotechnology (Lake Placid,NY).

Tg mice. Generation of IGF-II/IGF-I Tg mice has been described in detail elsewhere (Ye et al., 1996). They were bred as heterozygotesand maintained in a vivarium with 12 hr (light/dark) cycles at22°C. All procedures used were approved by appropriate committeesat the University of North Carolina at ChapelHill.

Brains from IGF-II/IGF-I Tg mice and their normal, non-Tg littermates were collected at P7, P14, and P21 (n $>=$ 5 for most experiments).Tg mice were identified by Northern hybridization analysis oftotal RNA prepared from the cerebral cortex (the transgene isexpressed in all brain regions at all postnatal ages), as previouslydescribed (Chrysis and Underwood, 1999). Briefly, 20 µg of totalRNA were electrophoresed in 1.2% formaldehyde-agarose gel, transferredto positively charged membranes, and UV cross-linked. Membraneswere hybridized with digoxenin-labeled RNA probes transcribedfrom the human IGF-I cDNA used in transgene, washed at high stringency,and detected by chemiluminescence. Transgene transcripts wereobserved in multiple sizes of ~2.8, 1.2, and 0.9 kb, as describedpreviously (Ye et al., 1996) and were much more abundant thanendogenous IGF-ImRNA.

Detection of apoptosis. Apoptotic cells in CB of Tg mice and their normal littermates were identified by terminal deoxynucleotidyltransferase-mediated deoxy-UTP nick end labeling (TUNEL), accordingto the manufacturer's instructions (Oncor, Gaithersburg, MD).Briefly, mice were perfused with 4% paraformaldehyde in 0.1 MPBS. The brainstem was transected in the transverse plane justrostral to the pons, and both the brainstem and CB were removedas a single piece. After paraffin embedding, serial sections werecut at a thickness of 5 µm, and every sixth section in the serieswas mounted on glass slides. Deparaffinized and rehydrated sectionswere treated with proteinase K (15 µg/ml) at 37°C for 10 min,and endogenous peroxidase activity was blocked with 3% hydrogenperoxide_. Slides were then placed in equilibrating buffer andincubated in a reaction buffer containing TdT and dUTP for 60min at 37°C. After rinsing, slides were incubated with peroxidase-conjugatedanti-digoxigenin (introduced together with Triton X-100 and ablocking agent). The sections were then exposed to 0.5 mg/ml diaminobenzidineand 0.05% hydrogen peroxide to generate a brown reaction productand covered with Crystal/Mount (Biomeda, Foster City, CA). Atleast six sections, 25 µg apart (to avoid counting the same cellstwice) were used to determine the number of apoptotic cells. Foreach section, cerebellar two-dimensional maps were traced usinga camera lucida. Completed maps were then digitized and measuredusing the Image-Pro image analysis system (Media Cybernetics,Silver Spring, MD). The number of apoptotic cells in each cerebellarsection was counted. Apoptotic cell number was expressed as afunction of cell density (cells per squaremillimeter).

RPA. Probe template cDNAs for mouse cyclophilin, Bcl-x, Bax, and Bcl-2 were purchased from Ambion. The Bcl-x riboprobe canprotect fragments of 60-80 nucleotide (nt) and 215 nt correspondingto Bcl-x short (Bcl-x_S) and long (Bcl-x_L), respectively. The Baxprotects a 167 nt fragment, Bcl-2 protects a 191 nt fragment,and the cyclophilin protects a 103 nt fragment. A mouse Bad cDNAof 419 bp was prepared by reverse transcription of mouse brainRNA, followed by amplification by PCR using primers designed accordingto the published sequence (Yang et al., 1995). The antisense primerwas 5'-CTAAGCTCCTCCTCCATCCC-3' (nucleotides 834-853), and thesense primer was 5'-AGGACTTATCAGCCGAAGCA-3' (nucleotides 434-453).The T3 promoter consensus sequence was linked to the 5'-end ofthe antisense primer, and the T7 promoter consensus sequence waslinked to the 5'-end of the sense primer. PCR yielded one fragmentat expected size that was then amplified and purified. Purifiedproduct was digested with the appropriate restriction enzymesto confirm its identity. Riboprobes were prepared by in vitrotranscription and purified on 5% acrylamide/8 M ureagel.

RPA was performed as reported previously (Chrysis et al., 1998). Briefly, 20 µg samples of CB total RNA were hybridized overnightat 45°C with biotin-labeled riboprobes (3 fmol of cyclophilin,2.5 fmol of Bcl-x and Bax, or 3 fmol of cyclophilin, 3 fmol ofBad, and 2 fmol of Bcl-2). After hybridization, samples were treatedwith A and T1 RNases, and protected fragments were separated in8% acrylamide/8 M urea gels and transferred to positively chargedmembranes by electroblotting. After washing, the signal was detectedaccording to manufacturer's recommendations (Ambion). Pilot experimentsusing constant amount of probes but different concentrations ofRNA confirmed that the concentration of probes was in molar excess.Yeast RNA hybridized with the above probes confirmed that thedigestion was complete. Bcl-x and Bax were studied in the samereaction because their protected bands can be easily distinguishedon the basis of size, and their abundances are similar. Protectedbands for Bcl-2 and Bad were much less abundant, requiring longerexposure times to develop their signals, and thus, they were studiedtogether in the same reaction. The signal for each protected bandwas normalized to that of cyclophilin and expressed as the ratioto the cyclophilinsignal.

Western immunoblot. Total protein extracted from the CB with the modified RIPA buffer (Tris-HCl 50 mM, pH 7.4, NP-40 1%, Na-deoxycholate0.25%, NaCl 150 mM, EDTA 1 mM, PMSF 1 mM, aprotonin, leupeptin,and pepsatin, 1 µg/ml each, Na₃VO₄ 1 mM, NaF 1 mM) was measuredaccording to the Bradford method (Bio-Rad, Hercules, CA). Equalamounts of proteins (30 µg for Bcl-x, Bax, Bad, and PARP; 40 µgfor caspase-3 at P7 and 60 µg at P14 and P21; and 120 µg for Bcl-2detection) were fractionated by 12% (or 8% for PARP) SDS-PAGEunder reducing conditions. Resolved proteins were electrophoreticallytransferred to PVDF membranes, blocked overnight at 4°C in NAP-Sure(Geno Technology, St. Louis, MO) diluted 1:1 in Tris-bufferedsaline (TBS; 10 mM Tris and 150 mM NaCl, pH 7.5). They were thenincubated with primary antibodies (antibodies against Bcl-x, Bad,Bax, PARP, and caspase-3 at 1:2000, and antibody against Bcl-2at 1:3500) in a 1:3 dilution of NAP-Sure/TBS at room temperaturefor 1 hr, washed in TBS with 0.1% Tween 20 several times, andincubated with horseradish peroxidase-conjugated anti-rabbit Ig(Transduction Laboratories, San Diego, CA) at 1:10,000 dilution.The antigen-antibody complexes were then detected by chemiluminescence.After development of films, blots were stained with Coomassieblue to assure equal loading of total protein. All experimentswere repeated at least twice using two different group ofmice.

Statistics. Data were calculated as means and SDs, and results were analyzed by Student's t test. p values <0.05 were consideredstatisticallysignificant.

  RESULTS

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ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Apoptosis during postnatal cerebellar development

To assess whether IGF-I overexpression alters apoptosis during cerebellar development, we used the TUNEL method to identifyapoptotic cells at P7, P14, and P21. At P7 IGF-I Tg mice had significantlyfewer apoptotic cells compared with their normal littermates (Fig.1; 35.4 ± 11.3 cells/mm² in Tg mice and 66.7 ± 6.7 in littermate controls; p < 0.01).At P14, Tg mice also exhibited a decrease in apoptotic cell number(16.0 ± 1.9 cells/mm² in Tg mice, compared with 37.5 ± 16.6 cells/mm² in controls), but the statistical significance was marginal (p= 0.09) because of the variability in normal littermates. Apoptoticcells were located mostly in the external granule layer (EGL).There were fewer apoptotic cells in the internal granule layer(IGL). Compared with P7 and P14, the number of apoptotic cellsat P21 was markedly decreased in both Tg and controls. Nonetheless,Tg animal tended to have fewer apoptotic cells (0.57 ± 0.2 cells/mm² in Tg mice, compared with 1.24 ± 0.5 cells/mm² in controls, p = 0.14). At this time, most apoptotic cells werelocated in the internal granule layer.

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Figure 1. Representative microphotographs from TUNEL assay in CBs from control (C) and IGF-I overexpressing transgenic (Tg) mouse at P7. CBs from P7 Tg animals had a 47% decrease in the number of apoptotic cells.

Caspases

Because caspases are thought to be the ultimate effectors of apoptosis in many situations, we investigated the abundance ofcaspase-3 to determine whether IGF-I modulates its expressionin the CB during early postnatal development. Western immunoblotsfor caspase-3 revealed that pro-caspase-3 was decreased in CBsfrom Tg mice at all ages studied, compared with normal littermates(Fig. 2 shows data from Tg mice expressed as a percentage of thatin normal, control mice). This finding was consistent in severalexperiments from different groups of mice. The decrease in pro-caspase-3in Tg mice does not reflect increased consumption of pro-caspase-3,however, because Tg mice also exhibited comparable decreases incaspase-3, the 20 kDa procaspase-3 cleavage product. More specifically,at P7 pro-caspase-3 was decreased by 59% in Tg mice (302 ± 42arbitrary units in Tg mice, compared with 512 ± 74 in controls;mean ± SD; p < 0.05), whereas the 20 kDa fragment was decreasedby 77% (120 ± 30, compared with 533 ± 111 in controls; p < 0.01);at P14 pro-caspase-3 was decreased 63.5% in Tg mice (343 ± 65,compared with 940 ± 137 in controls; p < 0.01), and the cleavageproduct was decreased by 68% (225 ± 53, compared with 571 ± 97in controls; p < 0.05); and at P21 these respective decreaseswere 60% (113 ± 46, compared with 286 ± 35; p < 0.05) and 52%(32 ± 6, compared with 67 ± 13; p < 0.05) (Fig. 2). During earlypostnatal cerebellar development, therefore, IGF-I overexpressionappears to decrease the expression of pro-caspase-3 without anapparent alteration in its activation, as judged by the relativeabundance of its cleavage product.

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Figure 2. Pro-caspase 3 (32 kDa) and its cleaved fragment caspase-3 (20 kDa) in Tg mice and their normal littermates during cerebellar development. A shows representative Western immunoblots from Tg mice and their normal littermates (controls) at P7, P14, and P21. B, Chemiluminescent signals were scanned for pro-caspase 3 (black bars) and its 20 kDa cleaved fragment (hatched bars) from P7, P14, and P21 Tg and control mice. For each developmental age studied, arbitrary optical density units for Tg mice are expressed as a percentage of control. Values represent the mean ± SD; *p < 0.05; **p < 0.01.

PARP

PARP, a 116 kDa protein, is a substrate for caspases and cleaved during apoptosis to an 85 kDa fragment. To obtain a measureof caspase activity, therefore, we assessed the abundance of PARPand its caspase-cleaved product. The abundance of 116 kDa PARPdecreased during normal cerebellar development (Fig. 3A). Therelative abundance of the 85 kDa fragment, however, was not concordantwith that of 116 kDa PARP, because its abundance was lower atP14 than at P7 and P21. The latter finding suggests that PARPis less actively cleaved at this time. The abundance of 116 kDaand 85-kDA PARP in Tg mouse CBs changes in a similar manner (Fig.3B).

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Figure 3. Changes in PARP abundance in Tg and normal mice during CB development, as assessed by Western immunoblot. A, Developmental changes of PARP (black bars) and its 85 kDa cleaved fragment (white bars) in CBs from control mice. Values represent the mean ± SD of arbitrary units derived from chemiluminescent signals. B, Developmental changes of PARP (black bars) and its 85 kDa cleaved fragment (white bars) in CBs from Tg mice. Values represent the mean ± SD of arbitrary units derived from chemiluminescent signals. *p < 0.05; **p < 0.01; ***p < 0.001.

Compared with normal controls, P7 Tg mice exhibited a 76% decrease in 85 kDa PARP fragment (p < 0.05) without a significantchange in the abundance of the uncleaved protein (Fig. 4A showsrepresentative Western blots, and B depicts the abundances of85 and 116 kDa PARP in Tg mice expressed as a percentage of thatin control mice). The ratio of 85 kDa to 116 kDa PARP in P7 Tgmice, therefore, was 25% (0.112 ± 0.015) of the ratio in controls(0.45 ± 0.03; p < 0.0001). This lower ratio in Tg mice is likelyto reflect decreased 116 kDa cleavage, and in turn decreased caspaseactivity. At P14 both the 85 kDa cleaved fragment and intact PARPwere significantly reduced in Tg mice (by 73 and 69%, respectively;p < 0.01), but the 85 to 116 kDa PARP ratio was not significantlyreduced (87% of control; 0.13 ± 0.016 in Tg mice and 0.15 ± 0.02in controls). At P21, both 85 kDa and 116 kDa PARP remained decreased(73 and 45% decreases, respectively), but the differences in the116 kDa PARP did not meet tests of statistical significance. Theratio of 85 to 116 kDa PARP, however, was reduced by 50% in Tgmice (5 ± 0.6), compared with controls (10 ± 1.6; p < 0.0001).These findings suggest that IGF-I overexpression reduces PARPexpression in the CB during development. In addition, it seemslikely that the decrease in the abundance of p85 kDa PARP relativeto that of 116 kDa PARP at P7 and P21 reflects reduced caspaseactivity.

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Figure 4. PARP protein from CBs of Tg and normal littermates, assessed by Western immunoblot. A shows representative Western immunoblots of 116 kDa PARP and its 85 kDa cleavage fragment in CBs from normal controls (C), and Tg mice at P7, P14, and P21. B, The abundance (mean ± SD) of PARP and its 85 kDa fragment in Tg CBs expressed as a percentage of that in their normal littermates. *p < 0.05; **p < 0.01.

IGF-I overexpression modulates the Bcl family of gene expression

The Bcl family of proteins, named for the prototype Bcl-2 gene, are intimately involved in the regulation of apoptosis. Bclproteins, such as Bcl-2 and Bcl-x_L, exert anti-apoptotic effects,whereas others have proapoptotic actions, e.g., Bax, Bad and Bcl-x_S.To determine whether IGF-I altered their expression in a mannerconsistent with IGF-I anti-apoptotic actions, we determined themRNA and protein abundance of Bcl family members with differentapparent actions on apoptosis. At each age studied during cerebellardevelopment, the expression of Bcl-2 and Bad (both mRNA and protein)was markedly less than that of Bcl-x and Bax. These differencesin abundance necessitated using different experimental conditions(e.g., differing exposure times for RPAs and differing amountsof proteins for western immunoblots) for each measure, and thus,only direct comparisons between Tg and normal CBs could be made,i.e., quantitative comparisons among Bcl proteins during developmentwere notpossible.

We obtained data on the expression of two anti-apoptotic Bcl family members, Bcl-2 and Bcl-x_L. Although the Bcl-x riboprobeused could detect both Bcl-x_L (a 215 nt band) and Bcl-x_S (60-80nt), no signals for the Bcl-x_S transcript were detected in eitherTg or normal mice at any age studied. Consistent with this finding,only the 29 kDa Bcl-x_L protein was detected by Western analysis.Compared with their normal littermates at P7 (Fig. 5), Bcl-x_LmRNA abundance was increased by 92% in Tg mice (0.27 ± 0.006 arbitraryunits, compared with 0.14 ± 0.01 in controls; mean ± SD; p < 0.001)and that of Bcl-x_L protein by 134% (2088 ± 314 arbitrary units,compared with 892 ± 183; p = 0.01; Fig. 6), whereas at P14 andP21 both mRNA and protein for Bcl-x_L were similar in Tg and theirnormal littermates (at P14: 0.25 ± 0.01 in Tg mice, compared 0.26± 0.01 in controls, p = NS, and 1749 ± 115 in Tg mice, comparedwith 1792 ± 308 in controls, p = NS, respectively; and at P21:0.405 ± 0.03 in Tg mice, compared with 0.451 ± 0.017, p = NS;and 1670 ± 78 in Tg mice, compared with 1931 ± 123 in controls,p = NS, respectively).

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Figure 5. Effects of IGF-I overexpression on Bcl-x_L Bcl-2, Bax, and Bad mRNAs assessed by RPA. A, Biotin-labeled gel-purified Bcl-x, Bax, and mouse cyclophilin riboprobes were cohybridized with 20 µg of total RNA from CBs. Each of the protested bands was of the expected size, i.e., 201, 167, and 100 nt, respectively. Bad, Bcl-2, and cyclophilin riboprobes also were cohybridized with 20 µg of total RNA giving bands of the expected sizes (491, 191, and 100 nt, respectively). B, Autoradiographic signals were scanned, normalized to those from cyclophilin, and expressed as a ratio of the signal to that of cyclophilin. Data (mean ± SD) from Tg mice is expressed as a percentage of their normal littermates. Hatched bars represent Bcl-2, white bars Bcl-x, black bars Bax, and cross-hatched bars Bad. *p < 0.05; **p < 0.01; ***p < 0.001.

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Figure 6. Effects of IGF-I overexpression on the Bcl-x_L, Bax, and Bad proteins assessed by Western immunoblot in CBs from P7, P14, and P21 Tg mice and their normal littermates. A shows representative Western immunoblots of Bcl-x, Bax, and Bad in CBs from Tg and normal (C) mice at P7, P14, and P21. B, Data (mean ± SD) from Tg mice is expressed as a percentage of their normal littermates. White bars represent Bcl-x, hatched bars Bax, and black bars Bad.

At P7 Bcl-2 mRNA abundance in Tg mice also was increased (72%; 0.1798 ± 0.013 arbitrary units, compared with 0.1043 ± 0.001;p < 0.01), but at P14 and P21 its abundance did not differ fromthat of control mice (0.168 ± 0.01 in Tg mice, compared with 0.148± 0.005 in controls, and 0.209 ± 0.010 in Tg mice, compared with0.206 ± 0.01, respectively; p = NS; Fig. 5). The abundance ofBcl-2 protein was very low in Tg and control CBs, and thus, quantificationwas not possible. At P7, however, Bcl-2 abundance appeared tobe increased in Tg mice. At P14 and P21 Bcl-2 protein was evenless abundant, and no differences could be discerned between Tgand normalCBs.

Changes in the expression of proapoptotic Bcl family members also were observed in Tg mice. At P7 Bax mRNA was increased by67% (0.066 ± 0.006 arbitrary units in Tg mice, compared with 0.04± 0.004 in controls; p < 0.01; Fig. 5), but Bax protein was unchanged(524 ± 68 in Tg mice, compared with 568 ± 103 in controls; p =NS; Fig. 6). At P14 Bax mRNA was unchanged (0.112 ± 0.01 in Tgmice, compared with 0.132 ± 0.005; p = NS), but protein abundancewas decreased by 35% in Tg mice (776 ± 125 in Tg mice, comparedwith 1187 ± 126; p < 0.05), whereas at P21 both Bax mRNA (0.185± 0.004 in Tg mice, compared with 0.245 ± 0.012; p < 0.01) andprotein abundance (913 ± 152 in Tg mice, compared with 3816 ±646; p < 0.01) were decreased in Tg mice (by 25 and 75%, respectively),compared with normallittermates.

Bad mRNA was increased by 43% in P7 Tg mice (0.600 ± 0.08 arbitrary units in Tg mice, compared with 0.391 ± 0.03; p < 0.05).Bad protein abundance was similar in Tg and normal mice (996 ±289 in Tg mice, compared with 902 ± 172; p = NS), but marked variationsin protein abundance were observed, especially in Tg mice. Infive different experiments from three different groups of mice,Bad protein was found to be either unchanged or moderately increased(by up to 35%) in Tg mice, but because of the high variabilityin Tg mice, these findings were not significant. Bad immunostainingat P7 revealed doublet bands. It is likely that one of these bandsrepresents phosphorylated Bad. The resolution of the doubletson our gels did not permit quantification of each separately.We, however, had the impression that the abundance of the lowerband was more variable and may have accounted for the variabilityof Bad abundance, especially in Tg CBs. At P14 Bad mRNA abundancewas decreased by 36% in Tg mice (0.48 ± 0.06 in Tg mice, comparedwith 0.68 ± 0.03; p < 0.05), and protein abundance was decreasedby 47% (441 ± 80 in Tg mice, compared with 803 ± 176; p = 0.036).At P21 Bad mRNA was decreased by 50% (0.093 ± 0.0020 in Tg mice,compared with 0.186 ± 0.017; p < 0.001) and protein by 62% (231± 45 in Tg mice, compared with 604 ± 74; p < 0.01). Doublet Badimmunostaining was not obvious at P14 and not observed atP21.

Our results demonstrate that IGF-I overexpression in the postnatal CB alters Bcl family gene expression in a developmentallyspecific manner. At P7 the abundance of each Bcl mRNA was significantlyincreased, but only Bcl-x_L protein abundance was increased, whereasat P14 and P21, Bax and Bad expression were decreased. Each ofthese changes is consistent with IGF-I anti-apoptotic actions,and changes in protein abundance are concordant with the inhibitionofapoptosis.

  DISCUSSION

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ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

We report that postnatal cerebellar IGF-I overexpression attenuates the apoptosis occurring in granule cells during cerebellardevelopment. Greater than 85% of the apoptotic cells identifiedwere in granule cell layers, and IGF-I inhibition of apoptosiswas similar in both the EGL and IGL. We believe that IGF-I derivedfrom Purkinje cells exerts anti-apoptotic actions directly ongranule cells, because the transgene (Ye et al., 1996), like thenative gene (Bondy and Lee, 1993), is expressed by Purkinje cellsand because IGF-I has been shown to inhibit apoptosis in primarycultures of granule cells (D'Mello et al., 1993; Leski et al.,2000). Our data, however, do not exclude indirect IGF-I effectson granule cells. IGF-I-induced decreases in apoptosis are associatedwith alterations in the expression of the Bcl family of proteins.Furthermore, altered Bcl expression occurs in a developmentallyspecific manner, such that in early postnatal life (P7) thereis increased expression of the anti-apoptotic genes, Bcl-x_L andBcl-2, whereas at later ages (P14 and P21) the expression of proapoptoticproteins, Bax and Bad, is decreased. These changes are associatedwith decreases in the expression of procaspase-3 and the activeenzyme, caspase-3, and decreased caspase-3 activity, as judgedby decreased abundance of the 85 kDa PARP cleavageproduct.

Between P5 and P9 of rodent cerebellar development, granule cells undergo a major wave of classical apoptosis, i.e., programmedcell death characterized by DNA fragmentation, (Landis and Sidman,1978; Wood et al., 1993). As judged by TUNEL, we found that postnatalcerebellar IGF-I overexpression attenuates apoptosis significantlyduring this time (P7). Inhibition of premitotic granule cellsapoptosis at P7 could result in a large increase in granule cellnumber, especially if all or most such cells subsequently undergoone or more rounds of division. Given that granule cell apoptosiswas decreased in throughout both the EGL and IGL of Tg mice, IGF-Ilikely inhibits apoptosis of both premitotic and in postmitoticcells. Our study, however, was not designed to address thisquestion.

Although not meeting tests of statistical significance, CBs from Tg mice had ~50% fewer apoptotic cells at P14 and P21. Anumber of other lines of evidence, however, strongly suggest thatIGF-I overexpression inhibits apoptosis at ages beyond the firstweek of postnatal development: (1) cerebellar overgrowth in IGF-ITg mice continues until adulthood, despite the fact that our previousstudies only detected evidence of small increases in granule cellproliferation (~10%) at one time during postnatal development(P15) (Ye et al., 1996); (2) the abundance of the 85 kDa fragmentof PARP, which can result from caspase cleavage during apoptosis,is significantly reduced in CBs from Tg mice at P21; (3) bothprocaspase 3 and its active fragment are significantly decreasedat P21, suggesting decreased apoptotic activity; and (4) the abundanceof the proapoptotic proteins Bax and Bad are significantly decreasedin CBs from Tg mice at P14 and P21. More detailed morphometricstudies will be necessary to determine the times when IGF-I anti-apoptoticactions have their greatest impact on granule cellnumber.

PARP synthesizes poly-ADP-ribose from nicotine amid dinucleotide in response to DNA strand breaks and is involved in manygenomic processes, including DNA base excision repair (Satoh etal., 1994) and DNA replication (Yoshida and Simbulan, 1994). PARPwas one of the first substrates shown to be cleaved by caspases.Although its role in apoptosis is not clear, a reduction in PARPcleavage can be taken as evidence of decreased apoptosis resultingfrom decreased caspase activity. Our findings of decreases inthe abundance of procaspase-3 and its activated enzyme at eachage studied are consistent with the latter speculation. A reductionin caspase activity, thus, could account for the decrease in cleavedPARP and represent a downstream mechanism for IGF-I anti-apoptoticactions. Relative to littermate controls, we found a decreasein cleaved PARP in the CBs of Tg mice at each time studied, aswell as decreased PARP expression at P14. We also observed thatPARP abundance decreased in normal mice during this period ofcerebellar development. The progressive decrease in PARP expression,therefore, also might be a reflection of the normal diminutionin cell proliferation, and consequently decreased requirementfor DNA repair, which occurs during the sameperiod.

At P7 before the expression of the IGF-I transgene has reached its peak [peak abundance occurs by ~P20 (Ye et al., 1996)],mRNA and protein abundances for the anti-apoptotic Bcl-2 and Bcl-x_Lare increased. The anti-apoptotic actions of Bcl-2 and Bcl-x_Lare well established in cultured neurons (Batistatou et al., 1993;Allsopp et al., 1993, 1995; de Luca et al., 1996) and in vivomodels (Martinou et al., 1994; Farlie et al., 1995; Gonzalez-Garciaet al., 1995; Motoyama et al., 1995; Michaelidis et al., 1996;Zanjani et al., 1996, 1997). We speculate, therefore, that theincrease of Bcl-2 and Bcl-x_L in CBs from Tg mice contributes tothe decreased apoptosis found in these mice at P7. The inductionof Bcl-2 and Bcl-x_L mRNAs and their proteins by IGF-I overexpressionis consistent with in vitro studies showing that IGF-I inducesBcl-2 promoter activation (Pugazhenthi et al., 1999) and expressionof the Bcl-x_L gene product in PC12 cells (Parrizas and LeRoith,1997). The upregulation of Bcl-2 and Bcl-x_L expression, however,appeared to be specific to the stage of development, because weobserved no difference between Tg and normal mice at P14 or P21.Although we have no explanation for the latter, it seems possiblethat the failure of IGF-I to increase Bcl-2 and Bcl-x_L expressionat later ages could reflect a compensatory mechanism. This speculationis consistent with the finding that IGF-I-induced Bcl-x_L expressionin cultured PC12 cells exhibits peaks 3 and 24 hr after IGF-Iexposure, but then declines (Parrizas and LeRoith, 1997).

Transcription of the Bcl-x gene generates two alternatively spliced mRNAs: a long form, termed BCL-x_L, which encodes a proteinwith anti-apoptotic activity, and a shorter form, Bcl-x_S, whichencodes a proapoptotic protein (Boise et al., 1993). The riboprobeused for RPAs and the antibody used in Western immunoblots eachrecognize both forms of Bcl-x. We, however, did not detect Bcl-x_Sin any experiment. This result is consistent with a report thatmouse tissues, including brain, do not express Bcl-x_S mRNA asjudged by both S1 nuclease protection assay and PCR (Gonzalez-Garciaet al., 1994).

The expression of the proapoptotic genes Bax and Bad also were affected by IGF-I, but in a manner different from Bcl-2 andBcl-x_L. At P7 IGF-I increased the mRNA abundance of both, buttheir protein abundance was not altered at this time, whereasat P14 and P21 IGF-I decreased the expressions of each in a mannerthat appeared to be progressive with time. Furthermore, the relativedecrease in protein abundance appeared greater than the decreasein mRNA abundance, suggesting the possibility of decreased mRNAtranslation or increased protein degradation. The increase ofBax and Bad mRNAs at P7 in Tg mice seems paradoxical in the viewof the IGF-I anti-apoptotic role. We speculate that this may representan adaptation to the increase in Bcl-2 and Bcl-x_L expression,rather than a direct effect of IGF-I overexpression. As mentionedabove, expression of the IGF-I transgene peaks at ~P20, the timewhen we observed a nadir in Bax and Bad expression. This patternleads us to speculate that higher IGF-I levels are necessary forIGF-I to modulate the expression of these proapoptotic proteins.Nonetheless, IGF-I actions on Bax and Bad expression may be crucialto its anti-apoptotic actions. Bax is clearly important in regulatingapoptosis in the CNS (Gillardon et al., 1995; Krajewski et al.,1995; Miller et al., 1997; Shindler et al., 1997; Vekrellis etal., 1997; Doughty et al., 2000; Selimi et al., 2000) and especiallyin cerebellar granule cells (Krajewski et al., 1995; Miller etal., 1997; Doughty et al., 2000; Selimi et al., 2000). For example,apoptosis after cerebral ischemia is associated with increasedBax expression in the CB (Doughty et al., 2000). Furthermore,cerebellar granule cells from Bax-deficient mice are resistantto apoptosis (Miller et al., 1997), and Bax deficiency in Lurchermice rescues granule cells from apoptosis (Doughty et al., 2000;Selimi et al., 2000).

Bad promotes cell death by binding to and blocking the anti-apoptotic activity of Bcl-x_L (Yang et al., 1995). When Bad isphosphorylated, it dissociates from Bcl-x_L, freeing Bcl-x_L toexert its activity as a suppressor of apoptosis. Phosphorylationof Bad takes place after activation of the PI3-K and its downstreamtarget, the serine-threonine kinase Akt (Datta et al., 1997; delPeso et al., 1997). IGF-I-induced neuronal survival has been linkedto the activation of the PI3-K pathway and the subsequent inactivationof Bad resulting from Akt phosphorylation (Datta et al., 1997).The antibody we used to detect Bad recognizes both phosphorylatedand nonphosphorylated forms, and it is likely that one of thedoublet bands noted on P7 Western blots represents phosphorylatedBad. The more slowly migrating band in the doublet was abundantin P7 CBs, but was not detected at P14 or P21. We suspect thatthis band represents phosphorylated Bad and that the high variabilitynoted in Bad protein levels at P7 in Tg mice are related to dynamicchanges in Bad isoforms induced by phosphorylation at this developmentaltime. A high proportion of phosphorylated Bad would also contributeto the significant reduction in apoptosis that occurs in P7 Tgmice. An antibody specific for phosphorylated Bad would providemore definitiveinformation.

Whereas IGF-I anti-apoptotic effects have been well documented in cultured cells, in vivo studies are few. A number of studiesindicate that intraventricular IGF-I administration can protectagainst neuron injury after hypoxia-ischemia (Guan et al., 1996,2000; Johnston et al., 1996), and Wang et al. (2000) demonstratedthat topical IGF-I application on the cerebral cortex can ameliorateapoptosis after ischemia. Recent evidence indicates that systemicallyadministered IGF-I can cross the blood-brain barrier (Armstronget al., 2000). Furthermore, systemically administered IGF-I appearscapable of protecting neuron from injury-induced apoptosis (Tagamiet al., 1997). Therefore, IGF-I appears capable of protectingagainst injury-induced neurondeath.

In summary, our data demonstrate that IGF-I attenuates apoptosis during cerebellar development by affecting multiple stepsin the apoptotic pathway in a developmentally specific manner.We believe that our data indicates an important role for IGF-Iin the normal control of apoptosis during CB development and thatit could be useful in the therapy of a variety of neural injuriesanddisorders.

  FOOTNOTES

Received Aug. 28, 2000; revised Nov. 28, 2000; accepted Dec. 5, 2000.

This work was supported by a Lawson-Wilkins Pharmacia & Upjohn Research Fellowship Award (D.C.) and by National Institutesof Health Grants HD08229 (A.J.D.) and DK-02506 (A.S.C.).
Correspondence should be addressed to Dr. A. Joseph D'Ercole, Department of Pediatrics, CB# 7220, University of North Carolina,Chapel Hill, NC 27599-7220. E-mail: joseph_d'ercole{at}unc.edu.

Dr. Chrysis' present address: Department of Woman and Child Health, Pediatric Endocrine Unit, Astrid Lindgren Children's Hospital,Q2: 08, Karolinska Institute, Stockholm, Sweden SE-17176.

  REFERENCES

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
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