Chronic oral L-DOPA increases dopamine and decreases serotonin excretions

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Chronic oral L-DOPA increases dopamine and decreases serotonin excretions

Néstor H. García, Theresa J. Berndt, Gertrude M. Tyce, and Franklyn G. Knox

Departments of Medicine and Physiology, Nephrology Research Unit, Mayo Clinic and Foundation, Rochester, Minnesota 55905

ABSTRACT

TOP
ABSTRACT
INTRODUCTION
METHODS
RESULTS
DISCUSSION
REFERENCES

Given the common pathways for uptake and synthesis for dopamine and serotonin, enhanced renal dopamine synthesis in responseto increased substrate 3,4-dihydroxyphenylalanine (L-DOPA) ispostulated to decrease renal serotonin synthesis. The presentstudy compared the effects of chronic oral administration of L-DOPAon dopamine and serotonin excretion in vivo, with the effectsof enhanced dopamine synthesis per nephron due to adaptation toreduced renal mass (RRM). Four groups of rats were studied: sham-operatedrats and rats with RRM in the absence and presence of chronicoral L-DOPA. L-DOPA (2 mg · 100 g body wt¹ · day¹) for 6-14 days increased calculated dopamine synthesis per nephronin sham-operated rats from 2.0 ± 0.3 (n = 7) to 13.6 ± 1.8 pg· day¹ · nephron¹ (n = 7, P < 0.05) and in rats with RRM from 6.1 ± 1.3 (n = 7)to 39.3 ± 5.2 pg · day¹ · nephron¹ (n = 7, P < 0.05). Chronic oral L-DOPA concomitantly decreasedserotonin synthesis per nephron in sham-operated rats (1.6 ± 0.1to 1.0 ± 0.1 pg · day¹ · nephron¹, n = 7, P < 0.05) and in rats with RRM (5.6 ± 0.9 to 2.6 ± 0.4pg · day¹ · nephron¹, n = 7, P < 0.05). Both serotonin and dopamine synthesis pernephron were increased in rats with RRM. In conclusion, chronicoral administration of L-DOPA enhances dopamine excretion anddecreases serotonin excretion in normal rats and in rats withreduced renal mass. Both dopamine and serotonin excretions pernephron were elevated by renal massreduction.

remnant kidney; rat; sodium; phosphate

	INTRODUCTION

TOP ABSTRACT INTRODUCTION METHODS RESULTS DISCUSSION REFERENCES

SYNTHESIS OF DOPAMINE and serotonin by the kidney from their precursors 3,4-dihydroxyphenylalanine (L-DOPA) and 5-hydroxytryptophan(5-HTP) occurs in the proximal tubules (10, 27). Uptake ofL-DOPA and 5-HTP by the proximal tubule cells occurs by the sametransporter (33), and both are decarboxylated by the enzymeL-aromatic amino acid decarboxylase (L-AADC) to produce dopamineand serotonin (10, 27). Given the common pathway for uptakeand synthesis, stimulation of the dopamine synthesis by increaseddelivery of substrate would be predicted to result in a decreasein serotonin synthesis. This notion is supported by in vitro studiesby Soares-da-Silva and colleagues (25, 26) but not by in vivostudies (15, 20).

Experiments performed in vitro using isolated rat renal proximal tubules demonstrated that L-DOPA interfered with inward transportof 5-HTP and also its decarboxylation by L-AADC in proximal tubulecells (25, 26). Isolated tubules were bathed with increasingconcentration of L-DOPA or 5-HTP ranging from 50 to 2,000 µM (25).L-DOPA was found to produce a concentration-dependent inhibitionof 5-HTP accumulation. These investigators also examined the interactionat the decarboxylation level of these two precursors. Incubationof proximal tubule cells with L-DOPA or 5-HTP resulted in a concentration-dependentincrease in formation of dopamine and serotonin, respectively,but when L-DOPA (5 µM) was added to the bath in the presence of5-HTP, serotonin synthesis was reduced by 30%. These two effectswould lead to increased synthesis of dopamine and decreased serotoninsynthesis by the proximal tubule, an effect that would be expectedto decrease in vivo serotoninexcretion.

In vivo studies by Itskovitz et al. (15) determined the renal effects of individual and simultaneous acute infusions ofL-DOPA and 5-HTP. In these studies, serotonin excretion was notaffected by L-DOPA infusion. Likewise, infusion of equimolar amountsof the kidney-specific precursors for dopamine and serotonin, $gamma$ -L-glutamyl-L-DOPA or $gamma$ -L-glutamyl 5-HTP in humans showed noevidence of competitive inhibition of synthesis of either amine(20).

A previous study demonstrated that rats with reduced renal mass (RRM) exhibit increased dopamine synthesis per nephron (12,13). However, the effect of RRM and the increased dopamine synthesisper nephron on renal serotonin synthesis has not been studied.Thus, in the present study, the effect on serotonin synthesisof increased dopamine synthesis per nephron in response to adaptationto RRM was compared with the effect of increased dopamine synthesisin response to increasedsubstrate.

	METHODS

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Male Sprague-Dawley rats, weighing 250-350 g, from Harlan Sprague Dawley (Indianapolis, IN) were used in thisstudy.

Surgical procedures were performed as follows. For the reduction of the renal mass, rats were anesthetized with an intramuscularinjection (0.1 ml/100 g body wt) of equal volumes of a solutionof xylazine (Lloyd Laboratories, 20 mg/ml) and ketamine hydrochloride(Ketalar, 100 mg/ml, Parke-Davis). Under aseptic and antisepticconditions, a right nephrectomy and surgical ablation of the leftrenal poles were performed. The adrenal glands were left intact.The amount of renal mass removed (in grams) was calculated byadding the weight of the right kidney to the weight of the removedleft kidney poles. The percentage of residual renal mass was thencalculated on the assumption that the right and left kidney werethe same weight and that each kidney contains 37,538 nephrons(17). Approximately 45% of the renal mass remained in rats thatunderwent RRM. This value was used to normalize the data per remainingnephron. Sham surgery was performed in another group of rats andthey served ascontrols.

After recovery from the anesthesia, rats were placed in the animal facility and allowed free access to water and food thesame night. Beginning the next day, all animals were pair-fed12 g/day of a diet containing 1.8% phosphate and 1% sodium. Foodintake was monitored to ensure that all food was consumed daily.L-DOPA (2 mg · 100 g body wt¹ · day¹) was added to the food. This dose of L-DOPA was previously shownnot to affect blood pressure (15).

Rats were divided in four groups: group 1, sham-operated rats (n = 7); group 2, rats with RRM (n = 7); group 3, sham-operatedrats treated with L-DOPA (n = 7); and group 4, rats with RRM treatedwith L-DOPA (n =7).

Rats were kept in metabolic cages, and urine was collected on the 6th, 10th, and 14th days after surgery and the initiationof L-DOPA. Twenty-four-hour urine samples were collected in acontainer in dry ice with the addition of 5 ml of 33% acetic acidand 0.5 ml of 1% cysteine to prevent dopamine and serotonin degradation.We determined dopamine, serotonin, sodium (Na⁺), potassium (K⁺) and phosphate (P_i)excretions.

Assays for urine measurements. Urinary free dopamine and serotonin were measured by the method of Tyce et al. (32). Briefly,0.1 ml of urine was diluted with 3 ml water, adjusted to pH 6.1,and applied to small columns (diameter 0.4 cm, height 2.3 cm)of Amberlite CG 50 (200-400 mesh). After washing the resin with3 ml of 2 mM phosphate buffer (pH 6.1) and 3 ml of water, catecholamineswere eluted with 5 ml of 0.2 M acetic acid. After the preliminaryextractions, compounds were quantitated by HPLC with electrochemicaldetection. Recoveries of added standards in all extractions averaged80-95%.

Sodium and potassium were measured with an IL943 Automatic Flame Photometer (Instrumentation Laboratory, Lexington, MA). Urinaryphosphate concentration was measured by the Chen method (3).

Statistical analysis. Data are reported as the mean for the 3 days that urine samples were collected. All data are reportedas means ± SE. Unpaired two-tailed t-test was used to determineif the changes observed were statistically significant, and P< 0.05 was accepted as a statistically significantdifference.

	RESULTS

TOP ABSTRACT INTRODUCTION METHODS RESULTS DISCUSSION REFERENCES

Because there were no significant differences in the results between the collections on days 6, 10, and 14, the data are presentedas the average values for the three 24-h urine collections. Absolutedopamine and serotonin excretions in untreated sham-operated orRRM rats and L-DOPA-treated sham-operated and RRM rats are shownin Table 1. Absolute dopamine excretions are similar in the untreatedsham-operated rats and RRM rats. Likewise, absolute serotoninexcretions are similar in sham-operated rats and rats with RRM.L-DOPA treatment significantly increased dopamine excretion insham-operated rats and rats with RRM. Absolute serotonin excretionsignificantly decreased in the L-DOPA-treated sham-operated ratsand rats with RRM.

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Table 1. Effect of chronic oral L-DOPA on dopamine and serotonin excretions in sham-operated rats and rats with RRM

Because rats with RRM had a reduced number of nephrons, Fig. 1 presents dopamine synthesis per nephron. As has been previouslyreported, rats with RRM have higher dopamine synthesis per nephronthan sham-operated rats (6.1 ± 1.3 compared with 2.0 ± 0.3 pg· day¹ · nephron¹). In the chronic L-DOPA-treated groups, dopamine synthesis pernephron increased to 13.6 ± 1.8 pg · day¹ · nephron¹ in sham-operated rats and to 39.3 ± 5.2 pg · day¹ · nephron¹ in RRM rats. Chronic L-DOPA treatment resulted in a sixfold increasein dopamine synthesis in the sham-operated rats as well as ratswith RRM. These high levels of dopamine synthesis were sustainedthroughout the experiment (data not shown).

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Fig. 1. Effect of reduction of renal mass (RRM) and chronic oral 3,4-dihydroxyphenylalanine (L-DOPA) on dopamine synthesis per nephron. Data are average of 3 days. Dopamine synthesis per nephron was enhanced within 6 days of RRM. L-DOPA administration increased dopamine synthesis. Sham, sham-operated rats (n = 7); Sham L-DOPA, sham-operated L-DOPA-treated rats (n = 7); RRM, rats with RRM (n = 7); RRM L-DOPA, rats with RRM and L-DOPA treated (n = 7). * Significant difference between untreated and L-DOPA-treated groups, P < 0.05. $ddager$ Significant difference between sham-operated rats and rats with RRM.

The effects of L-DOPA administration on serotonin synthesis per nephron in sham-operated rats and rats with RRM are summarizedin Fig. 2. As we observed with dopamine excretion, serotonin synthesisper nephron was increased in rats with RRM (5.6 ± 0.9 pg · day¹ · nephron¹) compared with sham-operated rats (1.6 ± 0.1 pg · day¹ · nephron¹). In the L-DOPA-treated groups, serotonin excretion decreasedto 1.0 ± 0.1 pg · day¹ · nephron¹ (P < 0.05) in sham-operated rats and to 2.6 ± 0.4 pg · day¹ · nephron¹ (P < 0.05) in rats with RRM. L-DOPA treatment decreased serotoninsynthesis by 50% in both groups.

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Fig. 2. Effect of RRM and chronic oral L-DOPA on serotonin synthesis per nephron. Data are average of 3 days. Serotonin synthesis per nephron was enhanced within 6 days of RRM. Chronic oral L-DOPA administration decreased serotonin synthesis per nephron. Sham, n = 7; Sham L-DOPA, n = 7; RRM, n = 7; RRM L-DOPA, n = 7. * Significant difference between untreated and L-DOPA treated groups, P < 0.05. $ddager$ Significant difference between sham-operated rats and rats with RRM.

Table 2 summarizes electrolyte excretion in sham and rats with RRM rats in the absence and presence of chronic oral L-DOPA.Phosphate excretion per nephron (U_{P_i}V/nephron) was twofold higherin the rats with RRM (142.6 ± 7.9 pM · day¹ · nephron¹) compared with sham-operated rats (67.5 ± 1.7 pM · day¹ · nephron¹). Phosphate excretion was 65.5 ± 2.3 pM · day¹ · nephron¹ in sham-operated rats treated with L-DOPA and 136.9 ± 4.8 pM· day¹ · nephron¹ in rats with RRM that received L-DOPA. Phosphate excretion didnot change with chronic administration of L-DOPA in either group(Table 2). Likewise, sodium (U_NaV/nephron) and potassium excretions(U_KV/nephron) were higher in rats with RRM, but chronic L-DOPAtreatment did not affect U_NaV or U_KV in either group.

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Table 2. Effect of chronic oral L-DOPA on electrolyte excretion in sham-operated rats and rats with RRM

	DISCUSSION

TOP ABSTRACT INTRODUCTION METHODS RESULTS DISCUSSION REFERENCES

The present study demonstrates that chronic oral L-DOPA treatment increases dopamine excretion and concomitantly decreasesserotonin excretion in normal rats and rats with RRM. Additionally,rats with RRM had higher dopamine and serotonin synthesis pernephron than their respectivecontrols.

In the kidney, serotonin is synthesized by the proximal tubule from its substrate 5-HTP (27). Because the rate of synthesisof serotonin is dependent on the availability of dietary tryptophan,which is a precursor for serotonin synthesis (6, 8, 30),all rats in the present study were fed the same amount of food.The enzyme L-AADC is not thought to be a rate-limiting step inthe synthesis of either serotonin or dopamine, because their synthesisis markedly increased by infusion of their substrates (15, 29).Although absolute serotonin excretions are not different betweenthe sham-operated and remnant kidney rats, it is important tonote that rats with a remnant kidney have a markedly decreasednumber of total nephrons. When serotonin excretion is expressedon the basis of the number of nephrons, serotonin synthesis pernephron is significantly higher in rats with RRM. Consistent withprevious studies (13), dopamine synthesis per nephron is alsoincreased in rats with a remnant kidney. Thus the intrarenal synthesisof serotonin and dopamine parallel each other after renal massreduction.

It is interesting to note that dopamine and serotonin excretions per nephron significantly increase within the first weekafter renal mass reduction (data not shown), and these levelswere sustained throughout the course of the experiment. This earlyincrease of dopamine and serotonin synthesis may accompany otherchanges such as an increase in growth factors (7), angiotensinogen(22), and other autacoids to achieve balance in this new condition.Thus the parallel increases in dopamine and serotonin synthesisper nephron represent enhanced metabolism by hypertrophied proximaltubulecells.

In agreement with the in vitro studies of Soares da Silva and Pinto-do (25), we found in vivo that chronic L-DOPA treatmentdecreased serotonin excretion. This effect was observed throughoutthe course of the experiment. However, the competition betweendopamine and serotonin synthesis by increased L-DOPA observedin vitro (25) and reported here in vivo was not reproduced inprevious in vivo studies using rats (15) or in humans (20).The in vivo studies by Itskovitz et al. (15) investigated therenal effects of individual and simultaneous acute infusion ofL-DOPA (76-380 nmol/min) and 5-HTP (341 nmol/min) to rats duringa period of 120 min. In contrast to our findings, excretion ofserotonin was not influenced by the concomitant administrationof L-DOPA. The reason for this difference may be related to thefact that they investigated the effect of L-DOPA and 5-HTP fora short period of time (2 h), whereas we collected urine for 24-hperiods during L-DOPAtreatment.

A lack of interaction between dopamine and serotonin synthesis was also observed by Li Kam Wa et al. (20) investigatingthe renal effects of the glutamyl derivative of L-DOPA (Glu-Dopa)in humans. In this study, the infusion of 18.7 µg · min¹ · kg¹ Glu-Dopa for 6 h was associated with a marked increase in dopamineexcretion, but serotonin excretion did not change. The reasonfor this difference may be related to the lower concentrationof infused L-DOPA compared with the present study. In agreementwith our findings, studies performed in patients with Parkinson'sdisease receiving L-DOPA reported that the urinary concentrationsof 5-hydroxyindoleacetic acid, a stable metabolite of serotonin,were decreased (31).

Dopamine excretion increased sixfold after oral L-DOPA administration and serotonin excretion decreased by 50%, whereas sodium,potassium, and phosphate excretions were not increased. This resultwas unexpected, inasmuch as several reports have demonstratedthat the acute intravenous or intrarenal infusion of dopamineor L-DOPA increased sodium (11) and phosphate (4, 5, 14,18) excretions. However, the effect of chronic oral administrationof L-DOPA on phosphate excretion has not been previously investigated.The lack of effect of chronic oral L-DOPA on sodium and phosphateexcretions in the present studies may be the result of severalmechanisms. First, it is possible that L-DOPA induces phosphaturiaand natriuresis only after infusion for a short period of time.This possibility is supported by the observation of Lederer etal. (19) in which dopamine inhibited phosphate transport inopossum kidney cells for only 3 h despite the continued presenceof dopamine in the media. Downregulation of dopamine receptorsmay also explain these results, and this suggestion is supportedby the observation of Song et al. (28) in vitro and Katayamaet al. (16) in rat kidneys. Both groups found that after 30days (28) and 15 days (16) of treatment with dopamine, thebinding sites for DA-1 receptors decreased, whereas DA-2 receptorswere unaffected. However, the possibility that binding changeswere followed by functional changes were not investigated in thesestudies. Decreased intrarenal synthesis of serotonin would bepredicted to be natriuretic and phosphaturic, because acute increasesin serotonin have been reported to enhance sodium and phosphatereabsorption in cultured proximal tubular cells (6, 8, 15,29). It is likely that downregulation of serotonin receptorsoccurs. Studies in opossum kidney cells demonstrated that incubationwith serotonin caused a desensitization of the functional responseafter 3 h followed by downregulation of the receptor (23). Alternatively,it is important to note that the natriuretic effect of dopamineis dependent on the experimental conditions (1, 9, 21,24), because previous studies demonstrated that the natriureticeffect of dopamine is evident in conditions of extracellular fluidvolume expansion but not in sodium-depleted states. It is unlikelythat the lack of natriuretic response to L-DOPA is due to sodiumdepletion, because in the present study all animals consumed asimilar normal sodium intake; however, the effect of L-DOPA wasnot determined in salt-loaded rats. Another less likely mechanismfor the lack of effect of increased dopamine synthesis on phosphateand sodium excretions is that dopamine may also bind $alpha$ - and $beta$ -adrenergicreceptors, which would increase sodium and phosphate reabsorption(2), thus any natriuretic and phosphaturic effects could beblunted by activation of the $alpha$ - and $beta$ -adrenergicsystem.

In conclusion, chronic oral administration of L-DOPA enhances dopamine excretion and decreases serotonin excretion in normalrats and in rats with RRM. Both dopamine and serotonin excretionsper remaining nephron were elevated by renal massreduction.

	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: F. G. Knox, Dept. of Physiology and Biophysics, Mayo Clinic and Foundation, 200 First St. SW, Rochester MN 55905 (E-mail: knox.franklyn{at}mayo.edu).

Received 16 February 1999; accepted in final form 16 July 1999.

	REFERENCES

TOP ABSTRACT INTRODUCTION METHODS RESULTS DISCUSSION REFERENCES

1. Agnoli, G. C., M. Cacciari, C. Garutti, E. Ikonomu, P. Lenzi, and G. Marchetti. Effects of extracellular fluid volume changes on renal response to low-dose dopamine infusion in normal women. Clin. Physiol. 7: 465-479, 1987[Medline].

2. Berndt, T. J., and F. G. Knox. Renal handling of phosphate. In: Textbook of Nephrology (3rd ed.). Baltimore, MD: Williams & Watkins, 1995, p. 388-398.

3. Chen, P., T. Toribara, and H. Warner. Microdetermination of phosphorus. Anal. Chem. 28: 1756-1758, 1956.

4. Cuche, J. L., G. R. Marchand, F. C. Greger, F. C. Lang, and F. G. Knox. Phosphaturic effect of dopamine in dogs. Possible role of intrarenally produced dopamine in phosphate regulation. J. Clin. Invest. 58: 71-76, 1976.

5. Debska-Slizien, A., P. Ho, R. Drangova, and A. D. Baines. Endogenous renal dopamine production regulates phosphate excretion. Am. J. Physiol. 266 (Renal Fluid Electrolyte Physiol. 35): F858-F867, 1994[Abstract/Free Full Text].

6. DeToledo, F. G., K. W. Beers, T. J. Berndt, M. A. Thompson, G. M. Tyce, F. G. Knox, and T. P. Dousa. Opposite paracrine effects of 5-HT and dopamine on Na⁺-Pi cotransport in opossum kidney cells. Kidney Int. 52: 152-156, 1997[Medline].

7. Grone, H. J., M. Simon, and E. F. Grone. Expression of vascular endothelial growth factor in renal vascular disease and renal allografts. J. Pathol. 177: 259-267, 1995[Medline].

8. Hafdi, Z., S. Couette, E. Comoy, D. Prie, C. Amiel, and G. Friedlander. Locally formed 5-hydroxytryptamine stimulates phosphate transport in cultured opossum kidney cells and in rat kidney. Biochem. J. 320: 615-621, 1996.

9. Hansell, P., and A. Fasching. The effect of dopamine receptor blockade on natriuresis is dependent on the degree of hypervolemia. Kidney Int. 39: 253-258, 1991[Medline].

10. Hayashi, M., Y. Yamaji, W. Kitajama, and T. Saruta. Aromatic L-amino acid decarboxylase activity along the rat nephron. Am. J. Physiol. 258 (Renal Fluid Electrolyte Physiol. 27): F28-F33, 1990[Abstract/Free Full Text].

11. Hegde, S. S., and M. F. Lokhandwala. Renal dopamine and sodium excretion. Am. J. Hypertens. 3: 78S-81S, 1990[Medline].

12. Isaac, J., T. J. Berndt, and F. G. Knox. Role of dopamine in the exaggerated phosphaturic response to parathyroid hormone in the remnant kidney. J. Lab. Clin. Med. 126: 470-473, 1995[Medline].

13. Isaac, J., T. J. Berndt, V. Thothathri, G. M. Tyce, and F. G. Knox. Catecholamines and phosphate excretion by the remnant kidney. Kidney Int. 43: 1021-1026, 1993[Medline].

14. Isaac, J., R. P. Glahn, M. A. Appel, M. Onsgard, T. P. Dousa, and F. G. Knox. Mechanism of dopamine inhibition of renal phosphate transport. J. Am. Soc. Nephrol. 2: 1601-1607, 1992[Abstract].

15. Itskovitz, H., Y. H. Chen, and C. T. Stier, Jr. Reciprocal renal effects of dopamine and 5-hydroxytryptamine formed within the rat kidney. Clin. Sci. (Colch.) 75: 503-507, 1988[Medline].

16. Katayama, E., T. Ogura, and Z. Ota. Characteristics of rat kidney dopamine receptors and the effects of renal denervation and dopamine infusion on these receptors. Nephron 53: 358-363, 1989[Medline].

17. Kaufman, J., H. J. DiMeola, N. J. Siegel, B. Lytton, M. Kashgarian, and J. P. Hayslett. Compensatory adaptation of structure and function following progressive renal ablation. Kidney Int. 6: 10-17, 1974[Medline].

18. LeClaire, M. M., T. J. Berndt, and F. G. Knox. Effects of renal interstitial infusion of L-DOPA on sodium and phosphate excretions. J. Lab. Clin. Med. 132: 308-312, 1998[Medline].

19. Lederer, E. D., S. S. Sohi, and K. R. McLeish. Dopamine regulates phosphate uptake by opossum kidney cells through multiple counter-regulatory receptors. J. Am. Soc. Nephrol. 9: 975-985, 1998[Abstract].

20. Li Kam Wa, T. C., S. Freestone, R. R. Samson, N. R. Johnston, and M. R. Lee. Renal metabolism and effects of glutamyl derivatives of L-DOPA and 5-hydroxytryptophan in man. Clin. Sci. (Colch.) 91: 177-185, 1996[Medline].

21. Muhlbauer, B., and H. Osswald. Urinary dopamine excretion in conscious rats: effect of carbidopa in different states of sodium balance. Renal Physiol. Biochem. 16: 117-124, 1993[Medline].

22. Olson, B. A., S. M. Ali, L. C. Contino, D. P. Brooks, and N. J. Laping. Angiotensin-converting enzyme inhibition alters clusterin mRNA expression in the kidney following renal mass reduction. Pharmacology 57: 13-19, 1998[Medline].

23. Pleus, R. C., and D. B. Bylund. Desensitization and down-regulation of the 5-hydroxytryptamine 1B receptor in the opossum kidney cell line. J. Pharmacol. Exp. Ther. 261: 271-277, 1992[Abstract/Free Full Text].

24. Ragsdale, N. V., M. Lynd, R. L. Chevalier, R. A. Felder, M. J. Peach, and R. M. Carey. Selective peripheral dopamine-1 receptor stimulation. Differential responses to sodium loading and depletion in humans. Hypertension 15: 914-921, 1990[Abstract/Free Full Text].

25. Soares-da-Silva, P., and O. P. Pinto-do. Antagonistic actions of renal dopamine and 5-hydroxytryptamine: effects of amine precursors on the cell inward transfer and decarboxylation. Br. J. Pharmacol. 117: 1187-1192, 1996[Medline].

26. Soares-da-Silva, P., M. A. Vieira-Coehlho, O. P. Pinto-do, M. Pestana, and A. M. Bertorello. Studies on the nature of the antagonistic actions of dopamine and 5-hydroxytryptamine in renal tissues. Hypertens. Res. 18: S47-51, 1995.

27. Sole, M. J., A. Madapallimattam, and A. D. Baines. An active pathway for serotonin synthesis by renal proximal tubules. Kidney Int. 29: 689-694, 1986[Medline].

28. Song, J. K., H. Cao, and X. L. Zhao. Renal D1 receptor, and not D2, are down regulated after long-term treatment with dopamine (Abstract). FASEB J. 11: A1329, 1997.

29. Stier, C. T., Jr., and H. D. Itskovitz. Formation of serotonin by rat kidneys in vivo. Proc. Soc. Exp. Biol. Med. 180: 550-557, 1985[Medline].

30. Tyce, G. M. Origin and metabolism of serotonin. J. Cardiovasc. Pharmacol. 16: S1-S7, 1990.

31. Tyce, G. M., M. D. Muenter, and C. A. Owen, Jr. Metabolism of L-dihydroxyphenylalanine by patients with Parkinson's disease. Mayo Clin. Proc. 45: 645-656, 1970[Medline].

32. Tyce, G. M., R. A. VanDyke, S. R. Rettke, S. R. Atchison, R. H. Wiesner, E. R. Dickson, and R. A. Krom. Human liver and conjugation of catecholamines. J. Lab. Clin. Med. 109: 532-537, 1987[Medline].

33. Vieira-Coelho, M. A., and P. Soares-da-Silva. Apical and basal uptake of L-DOPA and L-5-HTP and their corresponding amines, dopamine and 5-HT, in OK cells. Am. J. Physiol. 272 (Renal Physiol. 41): F632-F639, 1997[Abstract/Free Full Text].

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