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Department of Physiology and Biophysics, University of Mississippi Medical Center, Jackson, Mississippi 39216
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ABSTRACT |
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 TOP
 ABSTRACT
 INTRODUCTION
METHODS
RESULTS
DISCUSSION
REFERENCES
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Hepatic angiotensinogen secretion is controlled by a
complex pattern of physiological or pathophysiological mediators.
Because plasma concentrations of angiotensinogen are close to the
Michaelis-Menten constant, it was hypothesized that changes in
circulating angiotensinogen affect the formation rate of ANG I and ANG
II and, therefore, blood pressure. To further test this
hypothesis, we injected purified rat angiotensinogen intravenously
in Sprague-Dawley rats via the femoral vein and measured mean arterial
blood pressure after arterial catheterization. In controls, mean
arterial pressure was 131 ± 2 mmHg before and after the injection
of vehicle (sterile saline). The injection of 0.8, 1.2, and 2.9 mg/kg
angiotensinogen caused a dose-dependent increase in mean arterial blood
pressure of 8 ± 0.4, 19.3 ± 2.1, and 32 ± 2.4 mmHg,
respectively. In contrast, the injection of a purified rabbit anti-rat
angiotensinogen antibody (1.4 mg/kg) resulted in a significant decrease
in mean arterial pressure (
33 ± 3.2 mmHg). Plasma
angiotensinogen increased to 769 ± 32, 953 ± 42, and
1,289 ± 79 pmol/ml, respectively, after substrate and decreased
by 361 ± 28 pmol/ml after antibody administration. Alterations in
plasma angiotensinogen correlated well with changes in plasma renin
activity. In summary, variations in circulating angiotensinogen can
result in changes in blood pressure. In contrast to renin, which is
known as a tonic regulator for the generation of ANG I, angiotensinogen
may be a factor rather important for long-term control of the basal
activity of the renin-angiotensin system.
renin-angiotensin system; Sprague-Dawley rat; hypertension; plasma renin activity; anti-rat angiotensinogen antibody
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INTRODUCTION |
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TOP
ABSTRACT
INTRODUCTION
METHODS
RESULTS
DISCUSSION
REFERENCES
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THE RENIN-ANGIOTENSIN SYSTEMS both in blood and tissues (15, 20) are recognized as important effector systems for the regulation of blood pressure and salt and water homeostasis (8, 19). They have been implicated as a pathogenic factor in selected forms of primary or secondary hypertension (10, 16, 21). In the circulation, plasma concentrations of angiotensinogen are believed to directly influence the system's activity, because substrate concentrations are within the concentration range of the Km value of the substrate-enzyme reaction, which is, under most physiological or pathophysiological conditions, the rate-limiting step of the enzymatic cascade of the circulating renin-angiotensin system (1). The subsequent conversion of ANG I to active ANG II occurs rapidly and is generally not limiting because the angiotensin-converting enzyme is ubiquitously distributed. Several experimental findings confirmed the relationship between substrate and ANG I/ANG II formation. For example, selective knockout of angiotensinogen in mice (9) has been shown to decrease resting blood pressure in proportion to the number of alleles present in mice, and transfection of antisense oligonucleotides directed against exon 1 of the angiotensinogen gene induced a transient decrease in blood pressure in rats (24). In clinical studies of all components of the renin-angiotensin system, only mutations of the angiotensinogen gene have been reported to be associated with elevated blood pressure in humans, including the variants M235T and T174M (7, 14). These published findings on the genomic DNA, mRNA, or protein level support the hypothesis of a functional linkage between the expression of the substrate for renin and changes in blood pressure. However, until the present it was not clear how direct changes of substrate in the circulation on the protein level affect blood pressure. We have, therefore, in the current study injected physiological amounts of angiotensinogen in the Sprague-Dawley rat and monitored blood pressure changes. In addition, we analyzed how the observed changes in blood pressure are related to alterations in plasma concentrations of angiotensinogen and plasma renin activity.
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METHODS |
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TOP
ABSTRACT
INTRODUCTION
METHODS
RESULTS
DISCUSSION
REFERENCES
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Animals. Male Sprague-Dawley rats, body weight 300-350 g, were used in the experiments. Animals were kept under 24-h dark-light cycles, fed a standard rat chow, and had free access to water.
Animal instrumentation and blood pressure measurement. Blood pressure was measured in conscious chronically instrumented rats after catheterization of the femoral vein and carotid artery. Five days before experimentation, animals were anesthetized with isoflurane (4%) and surgically instrumented with a femoral venous (drug application) and carotid arterial (measurement of mean arterial blood pressure and blood withdrawal) catheter (PE-50) under aseptic conditions. Catheters were exteriorized at the nape of the neck and filled with heparin. The arterial line was connected to a pressure transducer and an oscillographic recorder (Grass, Quincy, MA), which records pulsatile and mean arterial pressure (MAP).
Experimental protocol for intravenous injections. The injection protocol was started after stabilization of blood pressure for 20-30 min. Subsequently, three different dosages (0.8, 1.2, and 2.9 mg/kg) of angiotensinogen were administered intravenously. Blood pressure was monitored for 45 min followed by the injection of 1.4 mg/kg of an anti-rat angiotensinogen antibody. Infusion volumes were 0.2-0.3 ml; sterile saline was used as vehicle. During the stabilization period, 30 min after the injection of angiotensinogen, and 10 min after antibody administration, 0.5-ml blood samples were taken for the analysis of plasma angiotensinogen and plasma renin activity.
Determination of plasma angiotensinogen. Angiotensinogen plasma concentrations were measured indirectly by quantitative conversion of angiotensinogen to ANG I with an excess of hog renin and subsequent radioimmunoassay of ANG I (18).
Determination of plasma renin activity. Plasma renin activity was measured after self-incubation of plasma at 37°C by an ANG I radioimmunoassay (3) using an antibody obtained from Chemicon (Los Angeles, CA).
Isolation of rat angiotensinogen. Rat angiotensinogen was isolated from plasma of nephrectomized rats according to a protocol described by Hackenthal and Hilgenfeldt in 1979 and 1980 (5). For improvement of the purity of the angiotensinogen preparation, an HPLC molecular weight column (GF-250, Zorbax) was added as an additional separation step. Angiotensinogen-containing fractions were detected by an indirect radioimmunoassay of ANG I (as described above) and by SDS-PAGE.
Anti-rat angiotensinogen antibody. Polyclonal antibodies against angiotensinogen were generated following a protocol of Vaitukaitis and colleagues (25). Antisera obtained after the last booster injection were subjected to protein A-Sepharose (Pharmacia, Piskataway, NJ) chromatography for isolation of the IgG fractions.
Statistics. Data represent means ± SE of three independent experiments. Mean values were compared by one-way ANOVA, repeated measures, and, if applicable, by Bonferroni's method.
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RESULTS |
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TOP
ABSTRACT
INTRODUCTION
METHODS
RESULTS
DISCUSSION
REFERENCES
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To clarify the importance of substrate concentrations for the
generation of ANG I/ANG II, we first injected varying amounts of
angiotensinogen intravenously into Sprague-Dawley rats subsequent to a
20- to 30-min control and adaptation period. During this time animals
had a MAP of 131 ± 2 mmHg. The administration of the vehicle, 0.3 ml sterile saline, did not significantly change MAP (data not shown).
The injection of 0.8, 1.2, or 2.9 mg/kg angiotensinogen resulted in
dose-related increases of MAP of 8 ± 1.4 (P 
0.05), 19.3 ± 2.1 (P 0.01), and 32 ± 2.4 mmHg
(P 0.005), respectively (Fig.
1). Maximum effects were obtained 30-40 min after intravenous administration of renin substrate. Subsequent to the clearance period, 45 min after substrate injection, blood pressure started to decrease in all experimental groups. At this
time rats of all three experimental groups were intravenously injected
with 1.4 mg/kg purified anti-rat angiotensinogen antibody. The
administration of the antibody resulted in a decrease of MAP by 28 ± 2.9, 37 ± 3.2, and 32 ± 3.9 mmHg in the experimental groups previously injected with 0.8, 1.2, or 2.9 mg/kg angiotensinogen, respectively. No significant differences were apparent between the
experimental groups with regard to the net decrease in blood pressure
after the injection of the same amounts of antibody (Fig. 1).
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To analyze whether the observed changes in blood pressure were
associated with alterations in circulating substrate, we determined plasma angiotensinogen concentrations. Before the injection of angiotensinogen, rats had plasma angiotensinogen concentrations of 683 ± 33, 695 ± 49, and 651 ± 53 pmol/ml in the three
experimental groups (Fig. 2) selected to,
subsequently, receive intravenous injections of 0.8, 1.2, or 2.9 mg/kg
angiotensinogen. After the injection of substrate, plasma
angiotensinogen concentrations increased to 769 ± 31 (P 0.05), 953 ± 42 (P 0.01), and
1,289 ± 79 pmol/ml (P 0.005), respectively (Fig. 2), 30 min after the administration of substrate. The injection of antibody
resulted in a significant (P 0.005) decrease in all
experimental groups to 463 ± 34, 652 ± 49, and 812 ± 48 pmol/ml
plasma, respectively (Fig. 2), as measured 10 min after the injection
of antibody.
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To evaluate whether the linkage between angiotensinogen plasma
concentrations and blood pressure has a functional impact on the
formation rate of ANG I/ANG II, we determined plasma renin activity in
the same plasma samples used to determine angiotensinogen concentrations. Plasma renin activities were 11.7 ± 1.2 (0.8 mg/kg angiotensinogen), 14.5 ± 1.8 (1.2 mg/kg
angiotensinogen), and 13.9 ± 2.1 ng ANG
I · ml
1 · h1 (2.9 mg/kg
angiotensinogen) before the injection of substrate. The intravenous
administration of angiotensinogen increased plasma renin activity to
14.7 ± 1.3 (P 0.1), 28.0 ± 3.5 (P 0.005), and 46.8 ± 3.1 ng ANG
I · ml1 · h1
(P 0.001), respectively, and the administration of
antibody resulted in a significant decrease (P 0.005) to 6.2 ± 1.4, 12.9 ± 2.0, and 26.4 ± 2.9 ng ANG
I · ml1 · h1, respectively
(Fig. 3).
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DISCUSSION |
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TOP
ABSTRACT
INTRODUCTION
METHODS
RESULTS
DISCUSSION
REFERENCES
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Renin-angiotensin systems in tissues and in the circulation play a critical role in blood pressure regulation and salt and water homeostasis (8, 15, 16, 19, 20). They have been discussed as a pathogenic factor in many forms of primary or secondary forms of hypertension. The starting point of the endocrine system is the prohormone of ANG I, angiotensinogen (23). Plasma angiotensinogen, synthesized in the liver and constitutively secreted into the circulation, has a plasma half-life of about 4-10 h. Angiotensin peptides derive from angiotensinogen by a series of proteolytic digestions. The rate-limiting step for the plasma renin-angiotensin system is, under most physiological or pathophysiological conditions, the cleavage of an inactive decapeptide (ANG I) from angiotensinogen by the aspartyl protease renin (4). This reaction is under the tonic control of the release of renin from secretory granules in juxtamedullary cells in the kidney. However, from a biochemical point of view plasma concentrations of angiotensinogen also directly influence the activity of the renin-angiotensin system, because substrate concentrations, in most species, are within the concentration range of the Km value of the enzyme-substrate reaction (1). This relation between angiotensinogen plasma concentration and ANG II formation is evident in several diseases and during pregnancy (2, 17). On a genetic level, several experiments are pointing toward the importance of angiotensinogen influencing the formation rate of ANG II and, therefore, blood pressure. Over- or underexpression of the angiotensinogen gene strikingly resulted in an increase or decrease of systemic blood pressure (9, 24). Most interestingly, blood pressure seems to be dependent on the number of alleles coding for angiotensinogen in the genome (9).
In accordance with these experimental studies are clinical observations that report an association of mutations in the angiotensinogen gene with elevated blood pressure (7, 14) or preeclampsia (6). With regard to blood pressure regulation, at present it is not clear how these identified mutations interfere with the kinetics of the cleavage reaction through renin, the rate-limiting step of the enzymatic cascade of the circulating renin-angiotensin system. However, in preeclampsia, the identified mutation (L10F) is part of the cleavage site identified by renin and causes changes in the kinetics of the cleavage reaction. Taken together, all the observed changes in angiotensinogen at the genomic or mRNA level in human and rat seem to support the hypothesis of a functional link between the expression of the substrate for renin and changes in blood pressure and its potential implication in the pathogenesis of hypertension in the spontaneously hypertensive rat and in humans. However, up to now nobody has addressed or confirmed the importance of circulating angiotensinogen protein for the adjustment of ANG II formation rate. This would be of importance because many physiological and pathophysiological factors are known to interfere with hepatic angiotensinogen secretion at the transcriptional or posttranscriptional level (1, 12). In a letter to the Editor, Menard and colleagues (13) mentioned that they observed an increase in blood pressure in rats on a low-salt diet. In rats on a regular diet they did not see a significant change in blood pressure after administration of the same dosage of angiotensinogen. The brief comment did not provide data on plasma renin activity. The dosage of 250 µg/rat used in their study may correspond to our lowest dosage, which resulted in very moderate increases in blood pressure, plasma concentrations of angiotensinogen, and plasma renin activity in rats on a normal diet. Because of the lack of critical information and because of the experimental and clinical evidence for an important role of substrate in the production of the vasoactive effector peptide ANG II, we have, therefore, in our current study addressed this issue in a greater detail. We injected angiotensinogen in various concentrations and monitored blood pressure changes, angiotensinogen plasma concentrations, and, most importantly, plasma renin activity. The injection of angiotensinogen dose dependently increased blood pressure in the Sprague-Dawley rat. Analysis of plasma angiotensinogen concentrations and plasma renin activity clearly indicated that the dosages used in the experiment correspond to plasma concentrations observed during various pathophysiological situations, such as nephrectomy or inflammation (11), or elevated glucocorticoid or estrogen plasma levels (10). In these studies plasma concentrations of angiotensinogen increased approximately two- or threefold subsequent to the administration of estradiol or dexamethasone, respectively. Nephrectomy usually results in 2- to 2.5-fold increases in plasma concentrations of angiotensinogen, and the administration of interleukin-6 led to a 2.5-fold increase. The highest amounts of angiotensinogen administered in our current experiments resulted in 1.8- to 1.9-fold increases in angiotensinogen plasma concentrations. These increases in circulating angiotensinogen are within the range of the changes observed in vivo. Results from our current study indicate a clear dose-response relationship between circulating angiotensinogen concentrations and mean arterial blood pressure. In addition, the administration of constant amounts of anti-rat angiotensinogen antibody resulted in similar decreases of blood pressure in all experimental groups independently of the amount of angiotensinogen injected before the administration of antibody. Our current data, therefore, indicate that changes (increase or decrease) in the amount of circulating angiotensinogen can indeed affect plasma renin activity and, therefore, blood pressure in the Sprague-Dawley rat.
Angiotensinogen secretion is sensitive to glucocorticoids, estrogens, mineralocorticoids, insulin, and glucagon (1, 10, 21). Additionally, inflammatory mediators, e.g., interleukin-1 or -6, as well as tumor necrosis factor, have been identified as regulatory elements (11, 22), although the role of angiotensinogen as an acute-phase protein is not clear at present. An important and well-recognized (12) positive-feedback regulator of angiotensinogen formation is the active peptide product, ANG II. This mechanism is believed to restore the plasma pool of angiotensinogen during pathophysiological situations of increased consumption of substrate and depends on a posttranscriptional (RNA stabilization) mechanism. Abnormalities of this important feedback mechanism may be involved in the pathophysiology of certain forms of primary or secondary hypertension. In the mouse, Kim and colleagues (9) reported an increase in blood pressure of ~8 mmHg per angiotensinogen gene copy, resulting in a difference of 16 mmHg between the two-copy and four-copy mouse while angiotensinogen plasma concentrations are elevated 1.45-fold. No data on plasma renin activity are available from this study. In our study we observed an increase in mean arterial blood pressure of 19 mmHg while plasma concentrations are elevated 1.4-fold after the injection of 1.2 mg/kg substrate. Our data seem to be comparable, at least for this dosage, to the effects observed in the mouse, although one has to anticipate different kinetics for the cleavage reaction in mice. The biochemical characteristics of both systems indicate that angiotensinogen is the rate-limiting factor in the mouse, while in the rat both renin and angiotensinogen are expected to be rate limiting.
In the rat as in the mouse, angiotensinogen has an influence on the formation rate of ANG I and ANG II. However, regulatory mechanisms for the generation of ANG II signaling through angiotensinogen production cannot be considered a very sensitive and tonic control of the system's activity because of the relatively long time lag needed for angiotensinogen secretion to respond to regulatory input. Such a role is recognized for renin, which is rapidly and effectively released from secretory granula. Angiotensinogen may rather play a role in mechanisms for long-term adjustment of the system's basic activity. Data from our current study demonstrate that acute changes in circulating angiotensinogen indeed have an effect on blood pressure regulation. Because, however, blood pressure regulation is a complex multifactorial process with considerable counterregulation to be anticipated, it is difficult to extrapolate long-term effects of elevated angiotensinogen plasma concentrations at this time. Future studies, including continuous infusions of angiotensinogen, remain to be done to address this important issue.
Perspectives
ANG II has been implicated in the etiology of genetic hypertension in humans and animals. Initial studies on the importance of the renin-angiotensin system, mostly conducted in dogs, led to the conclusion that renin is the only rate-limiting component in the enzymatic cascade. However, more recent studies on the genetic level indicated a strong association between mutations of the angiotensinogen gene and the pathogenesis of hypertension in rats and humans. In addition, cleavage kinetics for the enzyme-substrate reaction have been proven to be different in dogs compared with humans and rats. Our current study in rats demonstrated that the rate of formation of ANG I and ANG II is regulated in part by the availability of angiotensinogen, which is in accordance with the biochemical characteristics of the enzymatic cascade of the renin-angiotensin system. The current study used bolus injections of angiotensinogen to demonstrate its effect on blood pressure. Future studies remain to be done to address long-term effects of elevated angiotensinogen plasma concentrations on cardiovascular parameters to assess the importance of angiotensinogen for physiological blood pressure regulation and for the pathophysiology of several forms of primary and secondary hypertension.| |
ACKNOWLEDGEMENTS |
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This study was supported in part by Grant-in-Aid 9950874V from the American Heart Association, Southeast Affiliate (to C. P. R. Klett), by National Heart, Lung, and Blood Institute (NHLBI) Grant HL-33947 (to J. Granger), and by NHLBI Program Project Grant HL-51971.
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FOOTNOTES |
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Address for reprint requests and other correspondence: C. P. R. Klett, Dept. of Physiology and Biophysics, Univ. of Mississippi Medical Center, 2500 N. State St., Jackson, MS 39216 (E-mail: cklett{at}physiology.umsmed.edu).
The costs of publication of this article were defrayed in part by the payment of page charges. The article must therefore be hereby marked "advertisement" in accordance with 18 U.S.C. Section 1734 solely to indicate this fact.
Received 16 January 2001; accepted in final form 21 June 2001.
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REFERENCES |
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TOP
ABSTRACT
INTRODUCTION
METHODS
RESULTS
DISCUSSION
REFERENCES
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1.
Dzau, VJ,
and
Herrmann HC.
Hormonal control of angiotensinogen production.
Life Sci
30:
577-584,
1982[ISI][Medline].
2.
Eggena, P,
Hidaka H,
Barrett JD,
and
Sambhi MP.
Multiple forms of human plasma renin substrate.
J Clin Invest
78:
367-372,
1978.
3.
Haber, E,
Koerner T,
Page LB,
Kliman B,
and
Purnode A.
Application of a radioimmunoassay for angiotensin I to the physiologic measurements of plasma renin activity in normal human subjects.
J Clin Endocrinol Metab
29:
1349-1355,
1969[ISI][Medline].
4.
Hackenthal, E,
and
Taugner R.
Hormonal signals and intracellular messengers for renin secretion.
Mol Cell Endocrinol
47:
1-12,
1986[ISI][Medline].
5.
Hilgenfeldt, U,
and
Hackenthal E.
Purification and characterization of rat angiotensinogen.
Biochim Biophys Acta
579:
375-385,
1979[Medline].
6.
Inoue, I,
Rohrwasser A,
Helin C,
Jeunemaitre X,
Crain P,
Bohlender J,
Lifton RP,
Corvol P,
Ward K,
and
LaLouel JM.
A mutation of angiotensinogen in a patient with pre-eclampsia leads to altered kinetics of the renin angiotensin system.
J Biol Chem
279:
11430-11436,
1995.
7.
Jeunemaitre, X,
Soubrier F,
Kotelevtsev YV,
Lifton RP,
Williams CS,
Charru A,
Hunt SC,
Hopkins PN,
Williams RR,
Lalouel JM,
and
Corvol P.
Molecular basis of human hypertension: role of angiotensinogen.
Cell
71:
169-180,
1992[ISI][Medline].
8.
Johnston, CI.
Biochemistry and pharmacology of the renin-angiotensin system.
Drugs
39:
21-31,
1990.
9.
Kim, HS,
Krege JH,
Kluckman KD,
Hagaman JR,
Hodgin JB,
Best CF,
Jennette JC,
Coffman TM,
Maeda N,
and
Smithies O.
Genetic control of blood pressure and the angiotensinogen locus.
Proc Natl Acad Sci USA
92:
2735-2739,
1995
10.
Klett, C,
Ganten D,
Hellmann W,
Kaling M,
Ryffel GU,
Weimar-Ehl T,
and
Hackenthal E.
Regulation of hepatic angiotensinogen synthesis and secretion by steroid hormones.
Endocrinology
130:
3660-3668,
1992[Abstract].
11.
Klett, C,
and
Hackenthal E.
The response of hepatic angiotensinogen secretion to experimental inflammatory stimuli.
Agents Actions
38:
220-230,
1993[ISI][Medline].
12.
Klett, C,
Nobiling R,
Gierschik P,
and
Hackenthal E.
Angiotensin II stimulates the synthesis of angiotensinogen in hepatocytes by inhibiting adenylyl cyclase and stabilizing angiotensinogen mRNA.
J Biol Chem
268:
25095-25107,
1993
13.
Menard, J,
El Amrani AIK,
Savoie F,
and
Bouhnik J.
Angiotensinogen: an attractive and underrated participant in hypertension and inflammation.
Hypertension
18:
705-707,
1991
14.
Morise, T,
Takeuchi Y,
and
Takeda R.
Rapid detection and prevalence of the variance of the angiotensinogen gene in patients with essential hypertension.
J Intern Med
237:
175-180,
1995[ISI][Medline].
15.
Murakami, P,
Eggena P,
Barrett JD,
and
Sambhi MP.
Heterogeneity of renin substrate released from hepatocytes and in brain extracts.
Life Sci
34:
385-392,
1984[ISI][Medline].
16.
Nishimura, M,
Milsted M,
Bolck CH,
Brosnihan KB,
and
Ferrario CM.
Tissue renin-angiotensin systems in renal hypertension.
Hypertension
20:
158-167,
1992
17.
Novak, J,
Reckelhoff JF,
Bumgarner L,
Cockrell K,
Kassab SE,
and
Granger JP.
Role of nitric oxide in mediating the reduced sensitivity of the renal circulation to angiotensin II in pregnant rats.
Hypertension
30:
580-584,
1997
18.
Oster, H,
Hackenthal E,
and
Hepp R.
The renin angiotensin system.
N Engl J Med
291:
398-401,
1974.
19.
Reid, IA,
Morris BJ,
and
Ganong WF.
The renin angiotensin system.
Annu Rev Physiol
40:
377-410,
1978[ISI][Medline].
20.
Riordan, JF.
Angiotensin II: biosynthesis molecular recognition and signal transduction.
Cell Mol Neurobiol
15:
637-651,
1995[ISI][Medline].
21.
Samani, MJ.
Molecular biology of the renin-angiotensin system.
J Cardiovasc Pharmacol
18, Suppl 2:
S1-S6,
1991.
22.
Soden, M,
Klett C,
Hasmann T,
and
Hackenthal E.
Angiotensinogen: an acute phase protein?
Hypertension
23, Suppl:
I126-I130,
1994.
23.
Tewksbury, DA,
Frome WL,
and
Dumas ML.
Characterization of human angiotensinogen.
J Biol Chem
253:
3817-3820,
1978
24.
Tomita, N,
Morishita R,
Higaki J,
Aoki M,
Nakamura J,
Mikami H,
Fukamizu A,
Murakami K,
Kaneda Y,
and
Ogihara T.
Transient decrease in high blood pressure by in vivo transfer of antisense oligodeoxynucleotides against rat angiotensinogen.
Hypertension
26:
131-136,
1995
25.
Vaitukaitis, J,
Robbins JB,
Nieschlag E,
and
Ross GT.
A method for producing specific antisera with small dose of immunogen.
J Clin Endocrinol Metab
33:
988-991,
1976[ISI][Medline].
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