Angiotensin stimulates TGF-beta 1 and clusterin in the hydronephrotic neonatal rat kidney

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Angiotensin stimulates TGF- $beta$ 1 and clusterin in the hydronephrotic neonatal rat kidney

Kee Hwan Yoo¹, Barbara A. Thornhill², and Robert L. Chevalier²

¹ Department of Pediatrics, Korea University, Seoul, Korea 152-703; and ² Department of Pediatrics, University of Virginia, Charlottesville, Virginia 22908

ABSTRACT

TOP
ABSTRACT
INTRODUCTION
METHODS
RESULTS
DISCUSSION
REFERENCES

Unilateral ureteral obstruction (UUO) induces activation of the renin-angiotensin system and upregulation of transforminggrowth factor- $beta$ 1 (TGF- $beta$ 1; a cytokine modulating cellular adhesionand fibrogenesis) and clusterin (a glycoprotein produced in responseto cellular injury). This study was designed to examine the regulationof renal TGF- $beta$ 1 and clusterin by ANG II in the neonatal rat. Animalswere subjected to UUO in the first 2 days of life, and renal TGF- $beta$ 1and clusterin mRNA were measured 3 days later. Rats were dividedinto treatment groups receiving saline vehicle, ANG, losartan(AT₁ receptor inhibitor), or PD-123319 (AT₂ receptor inhibitor).ANG stimulated renal TGF- $beta$ 1 expression via AT₁ receptors, a responsesimilar to that in the adult. In contrast, clusterin expressionwas stimulated via AT₂ receptors, a response differing from thatin the adult, in which ANG inhibits clusterin expression via AT₁receptors. We speculate that the unique response of the neonatalhydronephrotic kidney to ANG II is due to the preponderance ofAT₂ receptors in the developingkidney.

AT₁ receptors; AT₂ receptors; losartan; PD-123319

	INTRODUCTION

TOP ABSTRACT INTRODUCTION METHODS RESULTS DISCUSSION REFERENCES

OBSTRUCTION TO URINE FLOW in early development impairs growth and maturation of the kidney and leads to nephron loss, tubularapoptosis, and interstitial fibrosis (7, 28). Chronic unilateralureteral obstruction (UUO) leads to profound changes in the renalexpression of a number of genes associated with cell proliferation,differentiation, and survival. These include marked stimulationof transforming growth factor- $beta$ 1 (TGF- $beta$ 1) and clusterin (6,10). In this study, we investigated the regulation of renalTGF- $beta$ 1 and clusterin expression after UUO in the neonatal rat.TGF- $beta$ 1 has been shown to upregulate clusterin expression and toinduce nuclear localization of clusterin (24, 35). Clusterinbinds to both type I and type II TGF- $beta$ receptors, but not theepidermal growth factor receptor, which is increased by neonatalUUO (30, 36).

TGF- $beta$ 1 is a cytokine that is produced in response to tissue injury and promotes cell-cell and cell-matrix contact (22, 45).Much attention has been focused recently on its role in fibrogenesis:TGF- $beta$ 1 stimulates cellular production of extracellular matrixcomponents, as well as inhibiting matrix degradation (37). Thusinhibition of TGF- $beta$ 1 reduces renal interstitial fibrosis, a majorlong-term consequence of chronic UUO (2). TGF- $beta$ 1 also stimulatescellular apoptosis, another deleterious renal consequence of chronicUUO (4, 6, 44).

However, TGF- $beta$ 1 also plays a salutary role in the cellular response to injury. By promoting extracellular matrix synthesisafter ischemic injury, TGF- $beta$ 1 provides regenerated tubular cellsa substrate for adhesion, migration, and exposure to ligands thatparticipate in the recovery process (3). In addition, TGF- $beta$ 1is a potent immunosuppressant: blocking TGF- $beta$ 1 expression couldaggravate the interstitial inflammatory response present as aresult of UUO (17).

Clusterin, a large glycoprotein also produced in response to tissue injury, plays a role in cellular aggregation and has beenassociated with protection from apoptosis (15) and shown toinduce aggregation of renal tubular cells in vitro (41). Bypreventing cellular detachment resulting from tubular injury,clusterin may reduce apoptosis activated by separation of thecell from its basement membrane, a process termed "anoikis" (16).In addition, clusterin plays a role in countering oxidant injury,which contributes to the renal damage resulting from UUO (39,51).

Chronic UUO also results in the stimulation of the renin-angiotensin system, which is already highly activated in the fetusand neonate compared with the adult (20). In addition to itsrole as a vasoconstrictor, ANG II has been shown to act as a growthfactor in the kidney, regulating both cellular proliferation andprogrammed cell death (apoptosis), depending on the distributionand subtype of receptors (43, 47). Thus stimulation of cellularproliferation is largely mediated by AT₁ receptors, whereas apoptosisor inhibition of proliferation is mediated by AT₂ receptors (43,47).

We and others (11, 23, 34) have shown that TGF- $beta$ 1 expression is regulated by ANG II, and that ANG-converting enzymeinhibitors or AT₁ receptor inhibitors reduce renal TGF- $beta$ 1 expressionby the hydronephrotic kidney and decrease interstitial fibrosis.We have also shown that inhibition of AT₁ receptors for 14 daysby losartan stimulates renal clusterin expression in the neonatalrat, suggesting that endogenous ANG II inhibits clusterin expressionthrough stimulation of AT₁ receptors (11). The present studywas designed to examine the regulation of TGF- $beta$ 1 and clusteringene expression by ANG II in the initial phase of UUO in the neonatalrat. A 3-day duration of UUO was used, as both AT₁ and AT₂ receptorsare abundant in the kidney at this age and renal AT₂ expressionfalls rapidly in the neonatal period (27, 48). Selective inhibitorsof AT₁ and AT₂ receptors were used to reveal their respectivecontribution, and exogenous ANG II was administered to additionalanimals to determine whether responses in gene expression couldbeelicited.

	METHODS

TOP ABSTRACT INTRODUCTION METHODS RESULTS DISCUSSION REFERENCES

Experiments were performed in 48 Sprague-Dawley rats, which were anesthetized with halothane and oxygen and subjected to UUOas described previously (11). Briefly, the left ureter was exposedthrough an abdominal incision, ligated, and the incision was suturedand the pup was returned to itsmother.

Rats were divided into eight groups (6 animals/group), as shown in Fig. 1. In four groups, the response of renal AT₁ receptorsto exogenous and endogenous ANG II was determined, whereas inthe remaining four groups, the response of AT₂ receptors was evaluated.Losartan (a gift of Merck, Rahway, NJ), a selective ANG II AT₁receptor inhibitor, was administered at 40 mg · kg¹ · day¹ by daily subcutaneous injection. This dose blocks the vasoconstrictorresponse to ANG II and is not toxic to rats receiving it overseveral months (46). PD-123319 (a gift of Parke-Davis, Ann Arbor,MI), a selective AT₂ receptor inhibitor, was administered usingtimed-release pellets (Innovative Research of America, Sarasota,FL) placed intraperitoneally at the time of ureteral obstruction.The pellets have been shown to release compounds reliably in severalstudies (13, 29, 42) and were manufactured to release PD-123319at 10 mg · kg¹ · day¹. This dose was chosen because chronic administration of PD-123319ranging from 3 to 30 mg · kg¹ · day¹ has been shown to have biological effects in rats (25, 26).Exogenous ANG II was administered using timed-release pellets(0.5 mg · kg¹ · day¹). Although we could not measure blood pressure in neonatal rats,this dose is nonhypertensive in adult rats (49) and would beexpected to be nonhypertensive in the neonate as well, in viewof the lower pressor response to ANG II in the neonate (40).Control rats received daily injections of saline vehicle, andrats not receiving PD-123319 or ANG II received placebo timed-releasepellets. Thus each animal received an identical number of injectionsand pellets.

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Fig. 1. Distribution of experimental groups. Top: 4 groups to determine role of AT₁ receptors in regulation of transforming growth factor (TGF)- $beta$ 1 and clusterin expression in neonatal hydronephrotic kidney. Bottom: 4 groups to determine role of AT₂ receptors in regulation of these genes. Los, losartan; PD, PD-123319.

Seventy-two hours after UUO, rats were killed by lethal injection of pentobarbital sodium. Kidneys were immediately removed,decapsulated, and processed for RNA analysis as described previously(11). Briefly, RNA was extracted using guanidinium isothiocyanate(9), and 10-µg samples were subjected to Northern blot analysisand hybridized with a rat TGF- $beta$ 1 cDNA (gift of Su Wen Quan, NationalCancer Institute, Bethesda, MD), clusterin cDNA (gift of M. Tenniswood,University of Ottawa, Ottawa, Ontario, Canada), and a 780-bp cDNAfragment of human glyceraldehyde-3-phosphate dehydrogenase (GAPDH;American Type Culture Collection, Rockville, MD). The latter wasused as a housekeeping gene to control for equal loading. Hybridizationsignals were determined by autoradiography and quantitated bydensitometry. The ratio of TGF- $beta$ 1 and clusterin mRNA to GAPDHmRNA was calculated for each kidney in eachgroup.

Statistical analysis. Data are presented as means ± SE. Comparisons between UUO and intact kidneys were made using the t-testfor paired data. The effects of exogenous ANG II and of AT₁ orAT₂ inhibitor were determined separately for UUO and intact oppositekidneys using one- and two-way ANOVA. Statistical significancewas defined as P < 0.05.

	RESULTS

TOP ABSTRACT INTRODUCTION METHODS RESULTS DISCUSSION REFERENCES

Mean body weight per rat pup ranged from 7 to 9 g and did not differ between groups. For all groups, renal TGF- $beta$ 1 expressionby the obstructed kidney exceeded that of the intact oppositekidney (see Fig. 3, A and B). This indicates that UUO inducesexpression of TGF- $beta$ 1 by the ipsilateralkidney.

As shown in Figs. 2 and 3, A and B, and Table 1, administration of exogenous ANG further increased renal TGF- $beta$ 1 expressionin the obstructed kidney, but not the intact opposite kidney.As revealed by two-way ANOVA (Table 1), this additional increasewas prevented by losartan but not by PD-123319. This indicatesthat exogenous ANG boosts the expression of TGF- $beta$ 1 in the obstructedkidney by binding to the AT₁ receptor. Administration of losartanminimally reduced the baseline renal expression of TGF- $beta$ 1 by boththe obstructed and intact opposite kidney (Fig. 3A, Table 1),whereas infusion of PD-123319 had no significant effect (Fig.3B, Table 1). This indicates that endogenous ANG stimulates TGF- $beta$ 1expression by binding to AT₁ receptors in both obstructed andintact opposite kidneys. It should be noted that by one-way ANOVA,TGF- $beta$ 1 expression was not different between ANG + PD-123319 andsaline treatment groups (Fig. 3B). This suggests that TGF- $beta$ 1 expressionmay also be stimulated by AT₂ receptors.

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Fig. 2. Representative Northern blots showing mRNA for TGF- $beta$ 1, clusterin, and glyceraldehyde-3-phosphate dehydrogenase (GAPDH). Shown are blots for 10 µg total RNA from kidneys of 2 rats from each group. UUO, kidney with ipsilateral unilateral ureteral obstruction; Intact, intact opposite kidney.

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Fig. 3. Relative renal TGF- $beta$ 1 and clusterin mRNA factored for GAPDH for each group. Relative renal TGF- $beta$ 1 mRNA expression: response to AT₁ receptor inhibition with losartan (A); response to AT₂ receptor inhibition with PD-123319 (B). Relative renal cluster in mRNA expression: response to AT₁ receptor inhibition with losartan (C); response to AT₂ receptor inhibition with PD-123319 (D). Data normalized for intact kidney saline group. Bars represent means ± SE (n = 5 or 6 rats/group); * P < 0.05 vs. intact kidney (paired t-test); ** P < 0.05 vs. saline-treated UUO kidney (1-way ANOVA).

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Table 1. Statistical comparison between treatment groups

As shown in Figs. 2 and 3, C and D, UUO alone did not affect ipsilateral renal clusterin expression, whereas ANG administrationsignificantly increased clusterin expression by the obstructedbut not the intact opposite kidney (Table 1). In contrast toits effect on TGF- $beta$ 1, losartan did not decrease the ANG-inducedstimulation of clusterin expression (Fig. 3C, Table 1). In contrast,PD-123319 prevented the response to exogenous ANG (Fig. 3D, Table1). This indicates that exogenous ANG boosts the expression ofclusterin in the obstructed kidney by binding to the AT₂ receptor.This effect of PD-123319 was greater after administration of exogenousANG than on baseline clusterin expression in the obstructed kidney(Fig. 3D, Table 1).

	DISCUSSION

TOP ABSTRACT INTRODUCTION METHODS RESULTS DISCUSSION REFERENCES

We previously reported that UUO in the neonatal rat causes a progressive increase in ipsilateral renal TGF- $beta$ 1 expression throughoutthe first month of life (10). The results of the present studyconfirm the stimulation of renal TGF- $beta$ 1 expression by UUO andreveal that a significant component of its expression is dependenton ANG II AT₁ receptors. A novel finding is the demonstrationof additional renal TGF- $beta$ 1 expression by exogenous ANG II in theobstructed kidney but not the intact opposite kidney. This indicatesthat the upregulation of TGF- $beta$ 1 by ANG II is enhanced in the obstructedkidney, an effect that occurs in the face of normalization ofreceptor expression after 3 days of UUO (48). One explanationfor this may relate to the demonstration of enhanced TGF- $beta$ 1 productionby stretching cultured mesangial cells, a response that is enhancedin the presence of ANG II (21). Because TGF- $beta$ 1 is also producedby tubular cells (1), which are stretched by tubular dilatationafter UUO, a similar mechanism may underlie our observations.Renal tubular cells express ANG AT₁ and AT₂ receptors, as wellas TGF- $beta$ receptors (1, 32, 33). In view of the lack ofeffect of 3 days of UUO on AT₁ and AT₂ receptor mRNA in eitherobstructed or contralateral kidneys (48), it is likely thatthese effects are mediated by signaling downstream from ANG bindingwith its receptors and modulated by the stretched tubules in theobstructedkidney.

We documented a linear correlation between the duration of UUO and renal mRNA expression of TGF- $beta$ 1 in the neonatal rat (10),and the intensity of tubular immunoreactive TGF- $beta$ 1 is also increasedin proportion to the duration of obstruction (8). In additionto its transcription and translation, activation of latent TGF- $beta$ 1also plays a role in its biological action. In this regard, ANGII not only stimulates the synthesis of latent TGF- $beta$ but alsopromotes its conversion to the biologically active form and increasesthe expression of type-1 TGF- $beta$ receptor (18, 19).

In light of the significant role played by TGF- $beta$ 1 in the progression of interstitial fibrosis, there is considerable interestin modulating its expression through regulation of ANG II. Wedemonstrated that 14 days of inhibition of AT₁ receptors withlosartan reduced TGF- $beta$ 1 expression in the obstructed neonatalrat kidney by 30%, without affecting expression in the intactkidney (11). Twenty-eight days after the relief of 5 days ofUUO in the neonatal rat, renal interstitial fibrosis was markedlyattenuated compared with the persistently obstructed kidney, whereasmicrovascular renin and tubular TGF- $beta$ 1 expression decreased significantly(8). ANG II has been shown to stimulate TGF- $beta$ 1 expression byrenal interstitial fibroblasts through AT₁ receptors and alsoto upregulate angiotensinogen in the fibroblasts themselves (38).We have shown that chronic administration of ANG II in the adultrat stimulates the expression of TGF- $beta$ 1 in glomeruli and tubulesand increases interstitial fibrosis (49).

We reported also that TGF- $beta$ 1 expression in the obstructed kidney of the neonatal mouse increased in animals with one to fourfunctional copies of the angiotensinogen gene, but not in thoselacking a functional angiotensinogen gene (14). Of interest,whereas the degree of renal interstitial fibrosis was directlyrelated to the number of copies of angiotensinogen (from 0 to2 copies), the reduction in fibrosis in mice without a functionalrenin-angiotensin system was only 50% (14). Moreover, usingin situ hybridization histochemistry, others have demonstratedincreased renal cortical interstitial TGF- $beta$ 1 mRNA and spontaneousinterstitial fibrosis in mice lacking functional copies of theangiotensinogen gene (31). These findings suggest that factorsother than ANG and TGF- $beta$ 1 also contribute to the progression ofinterstitialfibrosis.

We have shown that clusterin mRNA increases progressively throughout the first month of life in the neonatal rat kidney subjectedto UUO, whereas clusterin expression in the intact kidney remainsat baseline levels (5). Although renal clusterin expressionwas not stimulated by 3 days of UUO, clusterin was boosted additionallyby exogenous ANG II. The stimulation of renal clusterin expressionby ANG is a novel finding and is surprising in light of our previousreports showing stimulation of clusterin expression by losartanor enalapril in the obstructed or intact kidney of the 14-day-oldrat (11, 50). The present study shows clearly that the ANG-dependentstimulation of renal clusterin expression in 3-day-old rats wasmediated via the AT₂ receptors. Moreover, the response was limitedto the obstructed kidney. Immunoreactive clusterin follows thesame pattern, and relief of UUO at 5 days attenuates the distributionof clusterin-positive tubules at 1 mo of age (8). Thus thedistribution of the glycoprotein parallels the abundance of renalclusterinmRNA.

The stimulation of clusterin by ANG in the present study can be explained by a maturational shift in the balance between renalAT₁ and AT₂ receptors. At 1 day of age, the relative abundanceof renal mRNA for the AT₂ receptor is 10-fold greater than thatof the AT₁ receptor, whereas the distribution is virtually equalat 7 days (27). By 14 days, however, renal AT₂ receptor expressionhas decreased 30-fold below that of AT₁ receptors (27). We haveshown that renal AT₁ and AT₂ receptor binding correlates wellwith abundance of steady-state mRNA: as a result of 24 h of UUOin the neonatal rat, both AT₁ and AT₂ receptors are downregulatedin the obstructed kidney (48). However, by 3 days of UUO, renalAT₁ and AT₂ receptor expression is not different from that ofthe intact kidney, whereas by 28 days of UUO, AT₁ receptor mRNAand binding have increased compared with the intact kidney (48).Thus in the 3-day-old neonatal rat kidney, there is a preponderanceof AT₂ receptors, whereas in the 14-day-old animal, there is amarked preponderance of AT₁receptors.

As shown in the proposed scheme in Fig. 4, ANG II stimulates renal AT₂ receptors in the obstructed kidney of the 3-day-oldrat, resulting in upregulation of clusterin. PD-123319 blocksthis response, whereas losartan has no effect because of the relativepaucity of AT₁ receptors. In the 14-day-old rat, ANG II stimulatesthe more abundant renal AT₁ receptors, which attenuate clusterinexpression. Either losartan (which reduces AT₁ receptor activation)or enalapril (which reduces endogenous ANG II) increases renalclusterin expression in the 14-day-old rat by reducing the ANG-mediatedinhibition (11, 50). Although the magnitude is smaller, therenin-angiotensin system is activated by UUO in the adult as wellas in the neonate (6), and endogenous ANG would be expectedto reduce, rather than to stimulate, clusterin expression in theobstructed kidney. Thus, although ANG II clearly modulates renalclusterin expression, other factors are responsible for the primaryinitiation of clusterin upregulation after UUO.

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Fig. 4. Proposed scheme of effects of maturation on regulation of renal clusterin expression by ANG II. Relative abundance of ANG AT₁ and AT₂ receptors is denoted by size of circles. Left: relative distribution of renal ANG receptors in rats at 3 days of age; right: distribution in rats at 14 days through adulthood. Stimulation of AT₁ receptors downregulates clusterin, whereas stimulation of AT₂ receptors upregulates clusterin.

In summary, UUO in the neonatal rat activates the intrarenal renin-angiotensin system and induces the renal expression ofTGF- $beta$ 1 and clusterin. TGF- $beta$ 1 is upregulated through stimulationof the AT₁ receptors by endogenous or exogenous ANG II. Despitethe preponderance of renal AT₂ over AT₁ receptors in the firstweek of life and the shift to a preponderance of renal receptorsfrom AT₂ to AT₁ by the second week, ANG continues to stimulaterenal TGF- $beta$ 1 expression in the 14-day-old and adult rat, as itdoes in the first 3 days of life (11, 49). In contrast, inthe first 3 days of life, clusterin expression by the obstructedkidney is upregulated by exogenous ANG II through stimulationof the AT₂ receptors but not by AT₁ receptors. As reported byus previously, by the second week of life, ANG inhibits clusterinexpression by the obstructed kidney, an effect mediated by theAT₁ receptors (11).

Perspectives

We propose that the maturational shift in renal expression of ANG receptors from AT₂ to AT₁ explains the developmental changein regulation of renal clusterin expression by ANG II. The schemeproposed in Fig. 4 depicts opposing effects of ANG II bindingto AT₁ and AT₂ receptors. This paradigm has been established forother signaling pathways for AT₁ and AT₂ receptors. Thus vasoconstriction,sodium retention, and cell proliferation are mediated by AT₁ receptors(12). In contrast, vasodilatation and natriuresis (both throughthe generation of cGMP) or inhibition of cell proliferation andapoptosis are mediated by AT₂ receptors (12). In view of theubiquitous distribution of tissue renin-angiotensin systems, itis likely that the opposing signaling responses of AT₁ and AT₂receptors account for a number of maturational changes in theresponse toinjury.

	ACKNOWLEDGEMENTS

This research was supported in part by National Institute of Diabetes and Digestive and Kidney Diseases (NIDDK) Research Centerof Excellence in Pediatric Nephrology and Urology, DK-44756 andDK-52612; NIDDK O'Brien Center of Excellence in Nephrology andUrology, DK-45179; and National Institute of Child Health andHuman Development Child Health Research Center, HD-28810.

	FOOTNOTES

The costs of publication of this article were defrayed in part by the payment of page charges. The article must thereforebe hereby marked "advertisement" in accordance with 18 U.S.C.§1734 solely to indicate thisfact.

Address for reprint requests and other correspondence: R. L. Chevalier, Dept. of Pediatrics Box 386, Univ. of Virginia, Health Sciences Center, Charlottesville, VA 22908 (E-mail: rlc2m{at}virginia.edu).

Received 26 January 1999; accepted in final form 29 September 1999.

	REFERENCES

TOP ABSTRACT INTRODUCTION METHODS RESULTS DISCUSSION REFERENCES

1. Ando, T., S. Okuda, T. Yanagida, and M. Fujishima. Localization of TGF- $beta$ and its receptors in the kidney. Miner. Electrolyte Metab. 24: 149-153, 1998[ISI][Medline].

2. Ando, Y., Y. Isaka, M. Tsujii, Y. Akagi, Y. Kaneda, A. Yamauchi, A. Ando, N. Ueda, E. Imai, and M. Hori. Introduction of TGF- $beta$ antisense oligodeoxy-nucleotides into interstitial fibroblasts blocked tubulointerstitial fibrosis in unilateral ureteral obstruction rats (Abstract). J. Am. Soc. Nephrol. 9: 512A, 1998.

3. Basile, D. P., D. R. Martin, and M. R. Hammerman. Extracellular matrix-related genes in kidney after ischemic injury: potential role for TGF- $beta$ in repair. Am. J. Physiol. Renal Physiol. 275: F894-F903, 1998[Abstract/Free Full Text].

4. Bursch, W., F. Oberhammer, R. L. Jirtle, M. Askari, R. Sedivy, B. Grasl-Kraupp, A. F. Purchio, and R. Schulte-Hermann. Transforming growth factor- $beta$ 1 as a signal for induction of cell death by apoptosis. Br. J. Cancer 67: 531-536, 1993[ISI][Medline].

5. Chevalier, R. L. Growth factors and apoptosis in neonatal ureteral obstruction. J. Am. Soc. Nephrol. 7: 1098-1105, 1996[Abstract].

6. Chevalier, R. L., K. H. Chung, C. D. Smith, M. Ficenec, and R. A. Gomez. Renal apoptosis and clusterin following ureteral obstruction: the role of maturation. J. Urol. 156: 1474-1479, 1996[ISI][Medline].

7. Chevalier, R. L., S. Goyal, J. T. Wolstenholme, and B. A. Thornhill. Obstructive nephropathy in the neonatal rat is attenuated by epidermal growth factor. Kidney Int. 54: 38-47, 1998[ISI][Medline].

8. Chevalier, R. L., A. Kim, B. A. Thornhill, and J. T. Wolstenholme. Recovery following relief of unilateral ureteral obstruction in the neonatal rat. Kidney Int. 55: 793-807, 1999[ISI][Medline].

9. Chomczynski, P., and N. Sacchi. Single-step method of RNA isolation by acid guanidinium thiocyanate-phenol-chloroform extraction. Anal. Biochem. 162: 156-159, 1987[ISI][Medline].

10. Chung, K. H., and R. L. Chevalier. Arrested development of the neonatal kidney following chronic ureteral obstruction. J. Urol. 155: 1139-1144, 1996[ISI][Medline].

11. Chung, K. H., R. A. Gomez, and R. L. Chevalier. Regulation of renal growth factors and clusterin by angiotensin AT₁ receptors during neonatal ureteral obstruction. Am. J. Physiol. Renal Fluid Electrolyte Physiol. 268: F1117-F1123, 1995[Abstract/Free Full Text].

12. Chung, O., H. Kuehl, M. Stoll, and T. Unger. Physiological and pharmacological implications of AT1 vs. AT2 receptors. Kidney Int. 54, Suppl67: S95-S99, 1998.

13. Davidson, J. M., and K. N. Broadley. Manipulation of the wound-healing process with basic fibroblast growth factor. Ann. NY Acad. Sci. 638: 306-315, 1991[ISI][Medline].

14. Fern, R. J., C. M. Yesko, B. A. Thornhill, H.-S. Kim, O. Smithies, and R. L. Chevalier. Reduced angiotensinogen expression attenuates renal interstitial fibrosis in obstructive nephropathy in mice. J. Clin. Invest. 103: 39-46, 1999[ISI][Medline].

15. French, L. E., A. Wohlwend, A. P. Sappino, J. Tschopp, and J. A. Schifferli. Human clusterin gene expression is confined to surviving cells during in vitro programmed cell death. J. Clin. Invest. 93: 877-884, 1994.

16. Frisch, S. M., and H. Francis. Disruption of epithelial cell-matrix interactions induces apoptosis. J. Cell Biol. 124: 619-626, 1994[Abstract/Free Full Text].

17. Frishberg, Y., and C. J. Kelly. TGF- $beta$ and regulation of interstitial nephritis. Miner. Electrolyte Metab. 24: 181-189, 1998[ISI][Medline].

18. Fukuda, N., W.-Y. Hu, A. Kubo, M. Endoh, H. Kishioka, C. Satoh, M. Soma, Y. Izumi, and K. Kanmatsuse. Abnormal regulation of transforming growth factor-beta receptors on vascular smooth muscle cells from spontaneously hypertensive rats by angiotensin II. Hypertension 31: 672-677, 1998[Abstract/Free Full Text].

19. Gibbons, G. H., R. E. Pratt, and V. J. Dzau. Vascular smooth muscle cell hypertrophy vs. hyperplasia. Autocrine transforming growth factor- $beta$ 1 expression determines growth response to angiotensin II. J. Clin. Invest. 90: 456-461, 1992.

20. Gomez, R. A., K. R. Lynch, B. C. Sturgill, J. P. Elwood, R. L. Chevalier, R. M. Carey, and M. J. Peach. Distribution of renin mRNA and its protein in the developing kidney. Am. J. Physiol. Renal Fluid Electrolyte Physiol. 257: F850-F858, 1989[Abstract/Free Full Text].

21. Harris, R. C., Y. Akai, T. Yasuda, and T. Homma. Role of physical factors in the regulation of mesangial cell growth and the interaction with vasoactive agents. Exp. Nephrol. 2: 104, 1994[ISI][Medline].

22. Heino, J., R. A. Ignotz, M. E. Hemler, C. Crouse, and J. Massague. Regulation of cell adhesion receptors by transforming growth factor- $beta$ . J. Biol. Chem. 264: 380-388, 1989[Abstract/Free Full Text].

23. Ishidoya, S., J. Morrissey, R. McCracken, A. Reyes, and S. Klahr. Angiotensin II receptor antagonist ameliorates renal tubulointerstitial fibrosis caused by unilateral ureteral obstruction. Kidney Int. 47: 1285-1294, 1995[ISI][Medline].

24. Jin, G., and P. H. Howe. Regulation of clusterin gene expression by transforming growth factor- $beta$ . J. Biol. Chem. 272: 26620-26626, 1997[Abstract/Free Full Text].

25. Kuizinga, M. C., J. M. Smits, J. W. Arends, and M. P. Daemen. AT2 receptor blockade reduces cardiac interstitial cell DNA synthesis and cardiac function after rat myocardial infarction. J. Mol. Cell. Cardiol. 30: 425-434, 1998[ISI][Medline].

26. Levy, B. I., J. Benessiano, D. Henrion, L. Caputo, C. Heymes, M. Duriez, P. Poitevin, and J. L. Samuel. Chronic blockade of AT2-subtype receptors prevents the effect of angiotensin II on the rat vascular structure. J. Clin. Invest. 98: 418-425, 1996[ISI][Medline].

27. Mauch, T. J., G. Yang, E. Howe, K. M. Baker, and D. E. Dostal. Determination of renin-angiotensin system component mRNA levels in developing rat kidney using multiplex polymerase chain reaction (Abstract). J. Am. Soc. Nephrol. 8: 363A, 1997.

28. Medjebeur, A. A., L. Bussieres, B. Gasser, V. Gimonet, and K. Laborde. Experimental bilateral urinary obstruction in fetal sheep: transforming growth factor- $beta$ 1 expression. Am. J. Physiol. Renal Physiol. 273: F372-F379, 1997[Abstract/Free Full Text].

29. Nelson, K. G., T. Takahashi, N. L. Bossert, D. K. Walmer, and J. A. McLachlan. Epidermal growth factor replaces estrogen in the stimulation of female genital-tract growth and differentiation. Proc. Natl. Acad. Sci. USA 88: 21-25, 1991[Abstract/Free Full Text].

30. Nguyen, H. T., A. A. Thomson, B. A. Kogan, L. S. Baskin, and G. R. Cunha. Growth factor expression in the obstructed developing and mature rat kidney. Lab. Invest. 79: 171-184, 1999[ISI][Medline].

31. Niimura, F., P. A. Labosky, J. Kakuchi, S. Okubo, H. Yoshida, T. Oikawa, T. Ichiki, A. J. Naftilan, A. Fogo, T. Inagami, B. L. M. Hogan, and I. Ichikawa. Gene targeting in mice reveals a requirement for angiotensin in the development and maintenance of kidney morphology and growth factor regulation. J. Clin. Invest. 96: 2947-2954, 1995.

32. Ozono, R., Z. Q. Wang, A. F. Moore, T. Inagami, H. M. Siragy, and R. M. Carey. Expression of the subtype 2 angiotensin (AT2) receptor protein in rat kidney. Hypertension 30: 1238-1246, 1997[Abstract/Free Full Text].

33. Paxton, W. G., M. Runge, C. Horaist, C. Cohen, R. W. Alexander, and K. E. Bernstein. Immunohistochemical localization of rat angiotensin II AT₁ receptor. Am. J. Physiol. Renal Fluid Electrolyte Physiol. 264: F989-F995, 1993[Abstract/Free Full Text].

34. Pimentel, J. L., Jr., C. L. Sundell, S. S. Wang, J. B. Kopp, A. Montero, and M. Martinez-Maldonado. Role of angiotensin II in the expression and regulation of transforming growth factor- $beta$ in obstructive nephropathy. Kidney Int. 48: 1233-1246, 1995[ISI][Medline].

35. Reddy, K. B., G. Jin, M. C. Karode, J. A. K. Harmony, and P. H. Howe. Transforming growth factor- $beta$ (TGF- $beta$ )-induced localization of apolipoprotein J/clusterin in epithelial cells. Biochemistry 35: 6157-6163, 1996[Medline].

36. Reddy, K. B., M. C. Karode, J. A. K. Harmony, and P. H. Howe. Interaction of transforming growth factor- $beta$ receptors with apolipoprotein J/clusterin. Biochemistry 35: 309-314, 1996[Medline].

37. Roberts, A. B., B. K. McCune, and M. B. Sporn. TGF- $beta$ : regulation of extracellular matrix. Kidney Int. 41: 557-559, 1992[ISI][Medline].

38. Ruiz-Ortega, M., and J. Egido. Angiotensin II modulates cell growth-related events and synthesis of matrix proteins in renal interstitial fibroblasts. Kidney Int. 52: 1497-1510, 1997[ISI][Medline].

39. Schwochau, G. B., K. A. Nath, and M. E. Rosenberg. Clusterin protects against oxidative stress in vitro through aggregative and nonaggregative properties. Kidney Int. 53: 1647-1653, 1998[ISI][Medline].

40. Siegel, S. R. Decreased vascular and increased adrenal and renal sensitivity to angiotensin II in the newborn lamb. Circ. Res. 48: 34-38, 1981[Abstract/Free Full Text].

41. Silkensen, J. R., K. M. Skubitz, A. P. N. Skubitz, D. H. Chmielewski, J. C. Manivel, J. A. Dvergsten, and M. E. Rosenberg. Clusterin promotes the aggregation and adhesion of renal porcine epithelial cells. J. Clin. Invest. 96: 2646-2653, 1995.

42. Stagner, J. I., and E. Samois. The induction of capillary bed development by endothelial cell growth factor before islet transplantation may prevent islet ischemia. Transplant. Proc. 22: 824-828, 1990[ISI][Medline].

43. Tanaka, M., J. Ohnishi, Y. Ozawa, M. Sugimoto, S. Usuki, M. Naruse, K. Murakami, and H. Miyazaki. Characterization of angiotensin II receptor type 2 during differentiation and apoptosis of rat ovarian cultured granulosa cells. Biochem. Biophys. Res. Commun. 207: 593-598, 1995[ISI][Medline].

44. Tsukada, T., K. Eguchi, K. Migita, Y. Kawabe, A. Kawakami, N. Matsuoka, H. Takashima, A. Mizokami, and S. Nagataki. Transforming growth factor- $beta$ 1 induces apoptotic cell death in cultured human umbilical vein endothelial cells with down-regulated expression of bcl-2. Biochem. Biophys. Res. Commun. 210: 1076-1082, 1995[ISI][Medline].

45. Van Zoelen, E. J. J., and L. G. J. Tertoolen. Transforming growth factor- $beta$ enhances the extent of intercellular communication between normal rat kidney cells. J. Biol. Chem. 266: 12075-12081, 1991[Abstract/Free Full Text].

46. Wong, P. C., T. B. Barnes, A. T. Chiu, D. D. Christ, J. V. Duncia, W. F. Herblin, and P. B. M. W. M. Timmermans. Losartan (DuP 753), an orally active nonpeptide angiotensin II receptor antagonist. Cardiovasc. Drug Rev. 9: 317-339, 1991.

47. Yamada, T., M. Horiuchi, and V. J. Dzau. Angiotensin II type 2 receptor mediates programmed cell death. Proc. Natl. Acad. Sci. USA 93: 156-160, 1996[Abstract/Free Full Text].

48. Yoo, K. H., V. F. Norwood, S. S. El-Dahr, I. Yosipiv, and R. L. Chevalier. Regulation of angiotensin II AT₁ and AT₂ receptors in neonatal ureteral obstruction. Am. J. Physiol. Regulatory Integrative Comp. Physiol. 273: R503-R509, 1997[Abstract/Free Full Text].

49. Yoo, K. H., B. A. Thornhill, J. T. Wolstenholme, and R. L. Chevalier. Tissue-specific regulation of growth factors and clusterin by angiotensin II. Am. J. Hypertens. 11: 715-722, 1998[ISI][Medline].

50. Yoo, K. H., J. T. Wolstenholme, and R. L. Chevalier. Angiotensin-converting enzyme inhibition decreases growth factor expression in the neonatal rat kidney. Pediatr. Res. 42: 588-592, 1997[ISI][Medline].

51. Young, M. R. A., I. S. Young, S. R. Johnston, and B. J. Rowlands. Lipid peroxidation assessment of free radical production following release of obstructive uropathy. J. Urol. 156: 1828-1832, 1996[ISI][Medline].

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Angiotensin stimulates TGF-1 and clusterin in the hydronephrotic neonatal rat kidney

Angiotensin stimulates TGF- $beta$ 1 and clusterin in the hydronephrotic neonatal rat kidney