1 Hannah Research Institute, Ayr KA6 5HL, UK
2 Roslin Institute, Roslin, Midlothian EH25 9PS, UK
*Author for correspondence (e-mail: flintd{at}hri.sari.ac.uk)
Accepted 27 June 2002
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SUMMARY |
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Key words: IGFBP-5, Mammary gland, Involution, Apoptosis, Transgenic, Caspase, Plasmin, Mouse
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INTRODUCTION |
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This largely circumstantial evidence in support of an inhibitory role for IGFBP-5 is countered by a number of studies that have indicated an enhancing effect of IGFBP-5 on IGF-I action in vitro (Jones et al., 1993) and studies that have questioned the role of IGFBP-5 in prostate involution (Miyake et al., 2000
). Augmentation of IGF action typically involves proteolysis or reduction in the affinity of IGFBP-5 for IGF-1, often involving interaction with components of the extracellular matrix (Clemmons et al., 1998
; Nam, 2000
). We addressed aspects of this phenomenon in a recent study, in which we showed that, in the mammary gland, IGFBP-5 interacts with a milk protein,
s2-casein (Tonner et al., 2000
). Unlike its interaction with a number of other proteins or components of the extracellular matrix, the interaction of IGFBP-5 with
s2-casein did not reduce its affinity for IGF-I and thus its affinity remained in excess of that of the type I-IGF receptor. In addition, the study showed that IGFBP-5 concentrations in milk were in excess of 50 mg/l, which is several orders of magnitude greater than that of IGF-1. Typically, augmentation of IGF actions takes place when IGFBP and IGF are approximately equimolar but, when IGFBP concentrations are in excess, IGF actions are inhibited (Ewton et al., 1998
). Indeed, in all four transgenic mouse models described thus far (IGFBPs 1-4) growth inhibitory effects have been described (Murphy, 2000
).
In this study we sought to provide evidence for a causal relationship between IGFBP-5 and apoptosis by producing transgenic mice expressing IGFBP-5 from a mammary-specific promoter in order to examine various aspects of mammary development and function. These included histological analysis, measurement of caspase-3 (a marker of mammary apoptosis) (Marti et al., 2000; Marti et al., 2001
), plasmin activity (a marker of extracellular matrix degradation in the mammary gland) (Ossowski et al., 1979
; Busso et al., 1989
; Tonner et al., 2000
) pro-survival members of the Bcl-2 family and IGF signalling cascade. In this study we provide the first evidence that IGFBP-5 inhibits cellular proliferation and induces cell death, when expressed in the mammary gland of transgenic mice.
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MATERIALS AND METHODS |
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Production of IGFBP-5 transgenic mice
Production of transgenic mice was by injection of DNA into the pronuclei of fertilised eggs from superovulated F1 (CBA x C57B1/6) female mice mated with F1 stud male mice as described previously (Simons et al., 1987). The transgene rescue strategy (Clark et al., 1992
) was used, which involved the co-injection of the BLG transgene pSS1tgXS and pBJ69 containing the IGFBP-5 cDNA driven off BLG sequences. The IGFBP-5 cDNA (Shimasaki et al., 1991
) was inserted as a blunted EcoRI fragment into the EcoRV site of pBJ41 (Sola et al., 1998
). Transgenic mouse colonies were maintained on a mixed CBA x C57B1/6 background. Milk was collected at day 11 of lactation and processed as described (Simons et al., 1987
). Various tissues were taken from day 10 lactating mice to examine whether transgene expression was limited to the mammary gland. Mammary tissue samples were also obtained at days 10 and 15 of pregnancy and day 2 of lactation to compare the level of transgene expression at these times, using northern blotting.
Identification of transgenic mice
6- to 8-week old mice were anaesthetised with halothane and the tip of the tail removed for identification of the BLG transgene by PCR. DNA was extracted from tail biopsies using a Wizard ® Genomic Purification Kit (Promega, Southampton, UK) and resuspended in 10 mM Tris-HCl buffer containing 1 mM EDTA pH 8.0. Primer sequences for the transgene were 5'-GCT TCT GGG GTC TAC CAG GAA CCG-3' and 5'-GTC GTG CTT CTG AGC TCT GCA GGG-3'. Primers for acetyl-CoA carboxylase, which was used as a positive control were 5'-TCC GAG CTC GAT AAG AAG TGG GGA GGG AGA GCC-3' and 5'-TCC GAG CTC ACA CCA TAA GGT CAG AAA ATC TCC-3'. Oligonucleotides were synthesised by MWG Biotech UK Ltd (Milton Keynes, Bucks, UK). 24 µl of the following mix was added to 1.0 µl of DNA solution: 0.08 µl (0.4 U) of Taq DNA polymerase (Promega, Southampton UK), 2.5 µl of 10x buffer (supplied with enzyme), 0.25 µl of each oligonucleotide primer (25 pmoles of each), 1.0 µl of 25 mM MgCl2, 4.0 µl of deoxynucleotide triphosphate (dNTP) mix (1.25 mM each dATP, dCTP, dGTP and dTTP), 2 µl DMSO (8% final), and distilled water to bring the final volume to 24 µl. PCR amplification was performed as follows: 95°C for 1 minute, 30 cycles of 30 seconds at 92°C and 5 minutes at 65°C, then 5 minutes at 65°C. Amplified products were analyzed by electrophoresis through a 2% agarose gel.
Northern blotting
RNA was isolated from tissue using the RNAgents total RNA isolation system (Promega, Southampton, UK). 5 µg aliquots of RNA were separated by electrophoresis in 1.2% agarose gels containing 2.2 M formaldehyde and transferred to nylon membrane as described previously (Barber et al., 1992). Membranes were hybridised sequentially with cDNA probes to ovine ß-lactoglobulin and rat IGFBP-5 or an antisense riboprobe to murine ß-casein. The ovine ß-lactoglobulin probe was a 300 bp EcoRV-BamHI fragment of targeting vector pBJ41 (Sola et al., 1998
) corresponding to exons 5, 6 and 7 (3' UTR). The IGFBP-5 cDNA corresponded to a SacII-XhoI fragment within exon 1 of the rat cDNA (Shimasaki et al., 1991
). The ß-casein probe was an antisense riboprobe corresponding to nucleotides 55-382 of the mRNA (Yoshimura et al., 1986
). The hybridisation was performed as described previously (Barber et al., 1992
). The filters were exposed to a Kodak phosphor screen and the resulting images were scanned using a Molecular Dynamics (Sunnyvale, CA, USA) phosphorimager 445 SI.
Assessment of mammary development
Wild-type and transgenic dams were mated with male wild-type Tucks No 1 mice and checked for vaginal plugs to determine the day of mating (day 1 of pregnancy). Dams were killed by cervical dislocation on days 10 or 15 of pregnancy or on day 2 of lactation (parturition=day 1 of lactation). The 4th mammary gland was removed to prepare a whole mount for histological examination as described below. After photography portions of the whole mount were embedded in paraffin for sectioning and staining with Haematoxylin and Eosin. Glands were also frozen in liquid nitrogen for further analyses.
Assessment of lactation performance
All dams were mated with wild-type mice. At parturition, litters were adjusted to 8 in number. Pups were weighed daily to monitor growth and, if losses occurred, replacement pups were added to maintain litter size. In a second study, transgenic and wild-type dams were paired and their litters were exchanged on a daily basis to ensure that all of the effects on pup growth could be ascribed to the dam and not to her transgenic offspring. On day 10 of lactation the dams were killed by cervical dislocation and the second to fifth abdominal glands removed and weighed. Glands were either fixed for histological analysis as described below or stored in liquid nitrogen for determination of DNA content (Labarca and Paigen, 1980), acetyl-CoA carboxylase activity (the rate-limiting enzyme for de novo fatty acid synthesis) (Barber et al., 1992
), plasmin and plasminogen activities (Tonner et al., 2000
) and caspase-3 activity (R&D Systems Europe Ltd, Abingdon, UK). The caspase-3 assay was based on the hydrolysis of the peptide substrate acetyl-Asp-Glu-Val-Asp p-nitroanilide resulting in the release of the p-nitroaniline moiety. This was quantified spectrophotometrically at 405 nm. Tissues were homogenised in the lysis buffer provided (250 mM Hepes, pH 7.4, 1% Chaps, 50 mM DTT, 20 mM EDTA).
Treatment of transgenic mice with R3-IGF-I
Transgenic mice were mated and on day 8 of pregnancy were anaesthetised with halothane and a 100 µl osmotic minipump (Alza Corporation, Palo Alto, CA) was implanted subcutaneously in the interscapular region. The pump was designed to deliver 50 µg/day of R3-IGF-I (GroPep, Adelaide, Australia) in 0.1 M acetic acid for a period of 14 days, i.e. for the remaining period of pregnancy. At parturition litters were adjusted to 8 in number and weighed daily until dams were killed on day 10 of lactation.
Treatment of transgenic mice with GH
Transgenic mice were mated and from day 10 of pregnancy they received 300 µg of recombinant bovine GH (Monsanto) in 100 µl of 0.75% NaHCO3 daily until parturition. At parturition litters were adjusted to 8 in number and weighed daily until the dams were killed on day 10 of lactation. Mammary glands were removed and used, as indicated in the results, as well as for whole-mount analysis and histology.
Preparation of whole mounts of mammary gland
Individual mammary glands were placed on microscope slides, carefully spread with forceps and allowed to air dry for 10 minutes. They were then fixed in 10% formalin for 2-4 hours and washed in 70% ethanol for 15 minutes followed by a gradual change into distilled water. They were then stained overnight in a solution of 0.2% carmine, 0.5% aluminium potassium sulphate. After overnight staining, the gland was washed for 15 minutes in 70%, 95% and 100% ethanol before immersion in Histoclear for 5 minutes and finally mounting in DPX (VWR International, Poole, UK).
Histological analysis of mammary tissue
Mammary samples were fixed overnight in 4% paraformaldehyde, embedded in paraffin and 5-7 µm sections were cut and stained in Haematoxylin and Eosin.
Determination of IGFBP-5 concentrations in milk and serum
In order to verify co-integration of BLG and IGFBP-5, transgenic females were mated and, on day 10 of lactation, a milk sample was obtained as described previously. Milk samples were then examined for the presence of IGFBP-5 using the 125I-IGF-1 ligand blotting technique as described previously (Hossenlopp et al., 1986) and a radioimmunoassay for IGFBP-5 developed in our laboratory. Briefly, 125I-rIGFBP-5, IGFBP-5 standards and unknown samples, were incubated with a sheep antiserum to rIGFBP-5. After overnight incubation antibody-bound radioactive label was precipitated with an anti-sheep serum, centrifuged at 2000 g for 30 minutes, decanted, and the pellets, containing the antibody-bound IGFBP-5, counted in a gamma counter. The assay sensitivity was <15 ng/ml.
Proliferation studies
In the initial study mice received a single injection of bromodeoxyuridine (BrdU: 150 µl of 1 mg/ml) 2 hours before death on day 15 of pregnancy. In a second study mice were injected from day 16-20 of pregnancy, twice daily before killing on the day of parturition.
Mammary tissue was fixed in 4% paraformaldehyde, embedded in paraffin and sectioned at 4 µm. For the detection of BrdU incorporation, sections were pretreated with 50 µg/ml protease (S4508, Sigma, Dorset, UK) and any endogenous peroxidase activity was inhibited by treating with 2% (v/v) H2O2 in methanol for 10 minutes at room temperature. To denature the DNA the sections were incubated with 2 M HCl for 1 hour at 37°C. Sections were incubated with the primary antibody (M0744, DAKO, Cambridge, UK) diluted to 1:20 in 0.5% (w/v) bovine serum albumin in PBS for 1 hour and with the secondary antibody, antimouse biotinylated Ig, for 1 hour. Streptavidin biotin complex (K0377, DAKO, Cambridge, UK) was then applied to sections according to manufacturers instructions and the peroxidase activity was detected by incubating sections with a 0.5 mg/ml solution of 3',3-diaminobenzidine dihydrate (DAB). Cell nuclei were counterstained with Mayers Haematoxylin. Cells that stained positive for BrdU was quantified by using an image analysis system (Leica Q500MC, Nussloch, Germany) where at least 1000 nuclei per slide were counted from at least 6 separate fields. Results are represented as the percentage of cells that stained positive for BrdU.
Immunoblotting
Preparation of tissue homogenates, determination of protein concentrations and western immunoblotting was carried out exactly as described previously (Jeay et al., 2000). Uniformity of protein loading and transfer was confirmed by Ponceau Red staining of the membrane prior to blocking and incubation with antibodies. The antibodies used were, anti-IGF receptor (
-IR-3) (Oncogene Research Products, Boston, USA), diluted 1:1000, anti-Akt and anti-phospho-Akt (Cell Signalling Technology), diluted 1:1000, anti Bcl-2 and anti Bcl-xS/L (Santa Cruz Biotechnology Inc, USA) diluted 1:500. Secondary antibodies were peroxidase labelled anti-mouse or anti-rabbit, as appropriate (Amersham Pharmacia Biotech), diluted 1:5000 or 1:4000 respectively. Detection involved the enhanced chemiluminescence detection system of NEN Life Science Products Boston, US), according to the manufacturers instructions.
For determination of IGF-receptor phosphorylation, 250 µg of mammary gland supernatants were incubated overnight with anti-IR-3 antibody (diluted 1:1000). The primary antibody was then precipitated using protein A Sepharose (Amersham Pharmacia Biotech), the precipitate was washed extensively and then solubilised in Laemmli buffer before performing western blotting as described above using an anti-phosphotyrosine antibody (Upstate Biologicals, Lake Placid, US) diluted 1:4000 followed by an anti-mouse antiserum and detection by chemiluminescence as above. Quantification of bands was performed using Scion Image analysis.
Oligonucleosomal laddering
DNA was isolated from mouse mammary glands using the Wizard Genomic DNA Purification Kit according to the manufacturers instructions (Promega, Southampton, UK) and the DNA was quantified by fluorimetric assay (Labarca and Paigen, 1980). DNA was labelled by incubating 2 µg DNA in 100 mM Tris-HCl, pH 7.2, containing 10 mM MgCl2 with 100 nCi [32P]dCTP and 5 U of DNA polymerase (Klenow fragment) in a 50 µl volume at room temperature for 10 minutes. The reaction was stopped by adding EDTA (final concentration 10 mM), and the DNA was alcohol precipitated in the presence of ammonium acetate and 15 µg glycogen overnight at 80°C. DNA was recovered by centrifugation at (16,000 g), washed in 70% alcohol, air dried and resuspended in 10 mM Tris-HCl, pH 8.0, containing 1 mM EDTA. DNA (1 µg) was subjected to electrophoresis on 1.8% agarose gels in TBE with 5 µg/ml ethidium bromide. The gel was then fixed in 10% methanol/10% acetic acid, dried and exposed to a phosphorimage cassette and the image analysed by ImageQuant software (Molecular Dynamics, Sunnyvale, CA).
Statistical analysis
Growth curves were analysed using repeated measures ANOVA after adjustment for the lack of independence between errors using the Greenhouse-Geisser method. A more detailed analysis was performed by fitting logistic curves to derive slope, upper and lower asymptotes to permit us to undertake independent sample t-tests for wild-type versus transgenic mice. Where multiple comparisons were required, Fishers LSD test was used. For one data set REML was used because of imbalances in the data. In this case both the Wald test and the deviance were used to test for significance.
The remaining data was analysed by ANOVA with post-hoc testing by Fishers LSD.
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RESULTS |
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Pregnancy rates and litter size were unaffected in transgenic females (results not shown). However, immediately postpartum it was evident that these females showed impairment of lactogenesis (Fig. 3A). During the first 24-48 hours the pups failed to thrive and even after 48 hours, although pup weight gain increased, it did not reach the same rate as that of wild-type pups. Subsequently the glands of transgenic mice produced milk at around half the rate of wild-type animals suggesting some amelioration of the phenotype (Fig. 3A). Statistical analysis indicated that the rate of weight gain of pups (gradient of curve) at day 5 was significantly greater (P<0.001) for wild-type than transgenic dams. The delay in pup growth was also identified statistically by the fact that curve fitting revealed that the point of inflexion was significantly greater (P<0.01) for transgenic dams than for wild-type dams. Pup weight gain was significantly greater (P=0.006) for wild-type animals within 24 hours of birth. In order to rule out the possibility that transgenic pups developed abnormally, despite receiving normal amounts of milk from the transgenic dams, a second study was initiated in which litters were exchanged on a daily basis between wild-type and transgenic females. This study clearly showed that all litters failed to thrive during the periods spent with the transgenic dam but grew normally while with the wild-type dam (Fig. 3B). Again, statistical analysis revealed that the difference in growth rate of the pups when nursed by the wild-type or transgenic dams was highly significantly different (P=0.011). This conclusively demonstrated that the transgenic dams were failing to produce either sufficient quantity or quality of milk.
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We next addressed the question of the mechanism of action of IGFBP-5 by examining aspects of the IGF signalling cascade. The concentration of IGF receptor (IGFR) was unaffected in transgenic animals whereas IGFR phosphorylation was significantly impaired on day 1 but not day 10 of lactation (Fig. 11). Similarly, Akt levels were unaffected but phospho-Akt levels were significantly impaired on day 2 of lactation but not on day 10 (Fig. 11).
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DISCUSSION |
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Examination of the glands during pregnancy indicated that development was impaired, with reductions in both ductal branching, and alveolar end bud formation resulting in decreased invasion of the mammary fat pad and ultimately a decrease in the number of alveoli. At this time the alveolar epithelium is not fully polarised and tight-junctions are leaky suggesting that IGFBP-5 would have free access to the basolateral surfaces where IGF-I acts. This situation also pertains immediately postpartum (consistent with the greatly impaired milk production at this time). Within 24-48 hours however, tight junctions restrict apical-basal transport via this paracellular route (Nguyen and Neville, 1998; Nguyen et al., 2001
) and, since IGFBP-5 is secreted into milk, its biological effects are probably greatly attenuated. This would explain the recovery in pup weight gain that occurs around days 2-3 postpartum. The fact that these animals show only partial impairment of mammary development could reflect the fact that the transgene is expressed at relatively low levels during pregnancy and thus may not totally neutralise IGF bioavailability, or alternatively that compensatory mechanisms may exist to overcome the absence of IGF action in the mammary gland. Our data do not allow us to distinguish between these two possibilities.
When cellular function or alveolar integrity are compromised in the mammary gland, this is accompanied by an increase in caspase-3 activity (Marti et al., 2000; Marti et al., 2001
) and an increased conversion of plasminogen to plasmin (Ossowski et al., 1979
; Busso et al., 1989
; Tonner et al., 2000
). Both caspase-3 and plasmin activities were significantly increased on day 2 of lactation in transgenic mice providing strong evidence that expression of IGFBP-5 was able to promote inappropriate apoptosis and extracellular remodelling at this time similar to that which occurs during normal mammary involution (Marti et al., 2000
; Marti et al., 2001
; Ossoswksi et al., 1979
; Busso et al., 1987
; Tonner et al., 2000
). The demonstration of abnormal levels of caspase-3 and plasmin in early lactation, but normal levels of caspase-3 and plasmin on day 10 of lactation, adds further support to the proposal that the eventual closure of tight junctions prevents access of IGFBP-5 to the serosal side of the mammary gland, with a consequent loss of its apoptotic capacity between day 2 and day 10 of lactation. Both Bcl-2 and Bcl-xL are pro-survival molecules (Adams and Cory, 2001
) and, recently, conditional deletion of the Bcl-xL gene in the mammary gland has been shown to accelerate the rate of apoptosis (Walton et al., 2001
). Both Bcl-2 and Bcl-xL protein levels were decreased on day 1 of lactation consistent with increased cell death and we were able to confirm this by demonstrating an increase in the level of endonucleosomal ladder formation in the glands of IGFBP-5 transgenic mice at this time. Once again, the effects of the transgene were not apparent on day 10 of lactation, although in the case of Bcl-2 this was due to the fact that we were unable to detect Bcl-2 in either wild-type or transgenic animals at this time. These results are consistent with those of Metcalfe et al. (Metcalfe et al., 1999
) who demonstrated a loss of Bcl-2 expression in the mammary gland between pregnancy and day 9 of lactation. In addition these authors proposed that mammary epithelial cells are primed for apoptosis at parturition by de novo expression of Bak and Bad but that this is prevented by anti-apoptotic members of the Bcl-2 family. The decreased expression of two pro-survival Bcl family members in our transgenic animals adds weight to this hypothesis. The protection that IGF-I confers against apoptosis is known to occur through the activation of PI3-kinase and Akt, followed by phosphorylation-dependent inactivation of the proapoptotic protein Bad (Datta et al., 1997
). Our findings of altered levels of other Bcl-2 family members in IGFBP-5 transgenic animals adds further support to the importance of this pathway in cell survival.
We also provided evidence for reduced rates of cell proliferation around parturition but not on day 15 of pregnancy. It is our belief that the effectiveness of the transgene increases as its expression increases, in particular as parturition approaches. Its effects are probably maximal immediately postpartum when gene expression is high but tight junctions have not yet formed. Subsequently, when tight junctions close, the majority of the IGFBP-5 is secreted into milk rather than into the extracellular environment, with a subsequent loss of all of the phenotypic changes described. This may explain the partial rather than full impairment of mammary function.
Certain actions of IGFBP-5 have been proposed to occur independently of its ability to inhibit IGF action (Andress, 1998) and we therefore decided to examine whether IGF signalling was impaired by IGFBP-5 and to determine if R3-IGF-1, an analogue of IGF-1, could rescue the phenotype of the IGFBP-5 transgenic mouse. Clear evidence of impairment of IGF signalling was demonstrated by reduced phosphorylation of both the IGF receptor and reduced phosphorylation of Akt in IGFBP-5 transgenic mice. During involution of the mammary gland both the quantity and the phosphorylation status of the IGF receptor and Akt decrease (Hadsell et al., 2001
; Schwertfeger et al., 2001
). Furthermore Schwertfeger et al. (Schwertfeger et al., 2001
) demonstrated that constitutive expression of Akt could delay mammary involution. R3-IGF-I is an analogue that binds very weakly to IGFBPs (King et al., 1992
; Francis et al., 1992
) and we showed that this was able to completely overcome the effects of IGFBP-5 on mammary growth in terms of weight and DNA content but, whilst improving milk synthesis, it could not fully restore it. These findings suggest that IGF-I serves to promote proliferation and survival of mammary epithelial cells but that, at the same time, it impairs differentiation. Increased IGFBP-5 secretion has been associated with cellular differentiation in myoblasts (Rotwein et al., 1995
) and Schwann cells (Cheng et al., 1999
) although the nature of its role is under debate with studies suggesting stimulatory (Ewton et al., 1998
) or inhibitory (James et al., 1996
) effects of IGFBP-5 on IGF-I action. It is conceivable that the response of the cell is dependent upon the relative balance between IGFBP-5 and IGF-1. Thus, whilst an excess of IGFBP-5 results in cell death by neutralizing IGF-1 (as in natural involution or the IGFBP-5 transgenics) and an excess of IGF-1 results in mitogenesis and a lack of differentiation, a balance between the two may result in cell survival and differentiation. This hypothesis is currently under investigation in our laboratory and is supported by the studies of Ewton et al. (Ewton et al., 1998
) who showed concentration-dependent effects of IGFBP-5 in myoblasts with high concentrations inhibiting and lower concentrations augmenting differentiation.
In contrast, our attempts to mimic the effect of R3-IGF-I with GH (to stimulate endogenous IGF-I) failed to influence the phenotype of the transgenic animals. It is likely that GH could not increase IGF-I concentrations sufficiently to overcome the inhibitory effects of IGFBP-5. This is because IGFBP-5 is produced at concentrations that are several orders of magnitude higher than IGF-I, and GH treatment typically increases serum IGF-I concentrations by only two- to threefold in this model (Flint and Gardner, 1994). The results are also consistent with our failure to inhibit the involutionary process, after litter removal, using GH treatment (Tonner et al., 1997
). This contrasts with the effectiveness of prolactin in delaying involution, and could be explained by the observation that prolactin dramatically suppresses IGFBP-5 synthesis (Tonner et al., 1997
) which would enhance the effectiveness of endogenous IGF-I.
Although R3-IGF-I was very effective in stimulating mammary development, its failure to normalise milk yield might also reflect the fact that IGFBP-5 acts via an IGF-independent mechanism, acting through cell surface receptors of its own (Andress et al., 1998). We have also provided recent evidence that IGFBP-5 may act via an IGF-independent pathway involving interactions with plasminogen activator-inhibitor-1 (PAI-1) with resultant effects on tissue remodelling processes (Tonner et al., 2000
). However, we cannot rule out the possibility that, since the BLG promoter is active before day 10 of pregnancy, irreversible phenotypic changes may have been produced before IGF-treatment commenced.
This is the first report of a transgenic mouse expressing IGFBP-5. Overexpression of IGFBP-1 results in intrauterine and postnatal growth retardation (for a review, see Murphy, 2000). In order to address the issue of whether IGFBP-3 has augmentary or inhibitory actions, IGFBP-3 transgenic mice were produced using the phosphoglycerate kinase or cytomegalovirus (CMV) promoter (Modric et al., 2001
). Significant reductions in birthweight and postnatal growth were evident. Similarly, IGFBP-2, which has also been proposed as an enhancer of IGF effects, produced growth inhibition when expressed as a transgene on the CMV promoter, in growth hormone transgenic mice, which are double the normal size (Hoeflich et al., 2001
).
Whatever the precise mechanism of action of IGFBP-5, our study conclusively demonstrates, for the first time, that IGFBP-5 induces impaired mammary development and function when expressed at a concentration equivalent to that which occurs during physiological involution of the mammary gland and that this effect involves increased activity of caspase-3, and plasmin, as well as decreased concentrations of Bcl-2 and Bcl-xL. These findings are consistent with increased apoptotic cell death and extracellular matrix degradation. It also represents the first demonstration that neutralization of the effects of endogenous IGF-I results in impaired mammary gland development. This adds weight to the importance of IGF-I as a survival factor for the mammary gland (Hadsell et al., 1996; Neuenschwander et al., 1996
). Taken together these findings suggest that therapeutic approaches, which target inhibition of IGF action in the mammary gland, may prove successful, by mimicking a natural, physiological process. This process may not be limited to the mammary gland since IGFBP-5 is also expressed in association with apoptosis in a variety of tissues and at various developmental stages (see Allan et al., 2001
). We therefore propose that this represents a fundamental and generalised initiating event in the process of cell death and, as a consequence, control of IGF actions may have far reaching implications in cell biology.
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ACKNOWLEDGMENTS |
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