Pancreatic islet blood flow in conscious rats during hyperglycemia and hypoglycemia

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Pancreatic islet blood flow in conscious rats during hyperglycemia and hypoglycemia

M. Iwase, K. Tashiro, Y. Uchizono, D. Goto, and M. Yoshinari

Department of Medicine and Clinical Science, Graduate School of Medical Sciences, Kyushu University, Fukuoka 812 - 8582, Japan

ABSTRACT

TOP
ABSTRACT
INTRODUCTION
METHODS
RESULTS
DISCUSSION
REFERENCES

Anesthesia affects general hemodynamics and regulation of organ perfusion. We used colored microspheres to measure pancreaticislet blood flow in conscious rats at two time points, duringeither hyperglycemia or hypoglycemia. This method, using blackand green microspheres, was validated by comparison with previousmicrosphere experiments and by lack of effect of a nonmetabolizableglucose analog, 3-O-methylglucose, on islet perfusion. Basal andglucose-stimulated islet blood flow levels were similar in pentobarbitalsodium-anesthetized and conscious rats. However, the basal distributionof pancreatic blood flow was altered by anesthesia (fractionalislet blood flow 5.8 ± 0.4% in conscious rats, 7.9 ± 0.8% in pentobarbital-anesthetizedrats, P < 0.05). Insulin-induced hypoglycemia significantly increasedwhole pancreatic blood flow in conscious rats, whereas islet bloodflow remained unchanged and fractional islet blood flow was decreased(5.8 ± 0.5% in the basal state, 4.2 ± 0.4% during hypoglycemia,P < 0.001). Methylatropine pretreatment significantly increasedislet blood flow during hypoglycemia by 181%. This result suggeststhat prevention of hypoglycemia-induced increase in islet perfusionmay be mediated, at least in part, by a cholinergic, vagal muscarinicmechanism.

pentobarbital sodium; insulin; pancreas; methylatropine; microsphere

	INTRODUCTION

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REGULATION OF PANCREATIC ISLET perfusion is critical for the maintenance of metabolism of pancreatic islet cells as well asfor delivering islet hormones into the systemic circulation (3,10). In 1980, Lifson et al. (14) first measured islet bloodflow in anesthetized rabbits using a microsphere technique, andsimilar experiments were performed in anesthetized rats a fewyears later (12). Although anesthetic agents induce generalhemodynamic changes and alter regional perfusion regulation (19),measurement of islet blood flow in the nonanesthetized state hasnot previously been reported. In addition, anesthetic agents usedand the surgical stress involved in measurement procedures maythemselves elevate blood glucose levels and suppress insulin secretion(9). We therefore designed the present study to investigateregulation of islet perfusion in conscious rats. Both acute hyperglycemiaand insulin-induced hypoglycemia have been reported to cause apreferential increase in islet blood flow in anesthetized rats(12, 20). The former is mediated by the central nervous systemvia the vagus nerve (13) or by local nitric oxide release (16,21), whereas the mechanism of the latter has not yet been determined.In the present study, we investigated the effects of hyperglycemiaor hypoglycemia on islet blood flow in consciousrats.

Colored microspheres previously used for measurement of islet blood flow were of one color only (black) and thus allowed measurementof blood perfusion at one specific time point only (10). Becausevarious colored microspheres are now commercially available (6),we attempted to improve the measurement of islet blood flow usingdifferent colored microspheres in the sameanimal.

	METHODS

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Animals and surgery. Eight-week-old male Sprague-Dawley rats of ~300 g body weight (n = 55, Kyudo, Fukuoka, Japan) were used for the experiments.For anesthesia, pentobarbital sodium (Abbott Laboratories, Chicago,IL) was injected intraperitoneally at a dose of 50 mg/kg. Microsphereexperiments were performed in the anesthetized rats after stabilizationof blood pressure and body temperature. Body temperature was maintainedat 37.5°C using a body temperature controller (Fine Science Tools,Foster City, CA). Polyethylene tubing (PE-50) was implanted inthe ascending aorta via the right carotid artery, and the femoralartery was cannulated. Blood pressure was monitored by a pressuretransducer (Nihon Koden, Tokyo, Japan) connected to the arterialcatheter. Heparin (100 IU; Shimizu, Shizuoka, Japan) was administeredvia the right jugular vein. When conscious rats were used, theintravenous and arterial catheters were exteriorized through theback of the neck, filled with heparinized saline, and each wasplugged with a pin. Experiments were performed at least 72 h postoperatively.The microsphere experiments were performed in an unrestrainedstate after administration of heparin via the carotid catheterand stabilization of arterial blood pressure. All experimentswere performed according to the guidelines of the Animal ExperimentationEthics Committee of KyushuUniversity.

NEN vs. E-Z colored microspheres. Pentobarbital-anesthetized rats (n = 10) were used for comparison of two types of colored microspheres (NEN-TRAC microsphere,Du Pont, Wilmington, DE; E-Z TRAC microsphere, Interactive MedicalTechnology, San Diego, CA). NEN microspheres have been used previouslyfor measurement of islet blood flow in rats (10). Accordingto the information supplied by the manufacturers, the size distributionof NEN microspheres is 11.4 ± 0.1 (±SD) µm and that of E-Z microspheresis 10.0 ± 0.23 µm, and the density of NEN microspheres is 1.4g/ml, whereas that of E-Z microspheres is 1.05 g/ml. The latteris closer to the density of red blood cells (1.10 g/ml). NEN microspheresare black only, whereas E-Z microspheres are available in green,orange, red, blue, yellow, and black. Orange, red, and yellowE-Z microspheres were invisible in the blood reference sample,and black and blue microspheres were indistinguishable in pancreatictissue. Therefore, we used green and black microspheres in ourstudy. Black NEN microspheres and green E-Z microspheres wereused to compare NEN and E-Z microspheres. The order of administrationwas switched for every experiment. Islet blood flow was measuredaccording to the method of Jansson and Hellerström (12). Microsphereswere suspended in saline and sonicated before injection. Microspheres(400,000) were then injected and flushed with 350 µl saline intothe ascending aorta over 25 s. The reference blood sample waswithdrawn from the femoral artery catheter into a syringe at arate of 0.5 ml/min using a constant-withdrawal pump (model 120,KD Scientific, Boston, MA) commencing 10 s before injection ofthemicrospheres.

Blood samples were obtained for determination of blood glucose and serum immunoreactive insulin (IRI). Blood glucose was measuredby the electrode method (Glutest Ace, Kyotodaiichikagaku, Kyoto,Japan), and serum IRI was measured with an ELISA commercial kitusing a rat insulin standard (Morinaga, Yokohama, Japan). Therats were then killed, and the whole pancreas, entire duodenum,and adrenal glands were carefully removed, blotted, and weighed.The whole pancreas was carefully dissected free of fat and lymphnodes under a stereomicroscope (Leica MZ8, Leica, Heerbrugg, Switzerland).Each pancreas was cut into small pieces and placed between objectslides. Pancreatic specimens were treated with a freeze-thawingtechnique to facilitate visualization of microspheres and pancreaticislets. The volume of the islets as a percentage of the pancreatictissue was determined using the point-counting method (4).Intersections of overlapping islets were counted at a magnificationof ×40, and a total of 36 ± 1 different fields was counted ineach pancreas (corresponding to 4,329 ± 79 points; n = 55). Wholepancreas and duodenum were digested overnight with 2 mol/l NaOHat 70°C. The microsphere content of each organ and reference bloodsample were determined by transferring parts of the samples, aftervigorous stirring, to glass microfiber filters (GF/A, Whatman,Kent, UK) and counting the microspheres under a stereomicroscope.By determining the number of microspheres present in the organand arterial reference samples, blood flow values were calculatedaccording to the formula Q_org = N_org × 0.5/N_ref, where Q_org isthe organ blood flow (ml/min), 0.5 is the withdrawal rate of thereference sample (ml/min), N_org is the number of microspheresin the organ, and N_ref is the number of microspheres in the referencesample. A difference of <10% in microsphere content of the twoadrenal glands was taken to indicate sufficient arterial mixingof microspheres. When the islet blood flow was expressed per isletweight, islet weight was estimated by multiplying the pancreaticweight by the islet volume fraction of the whole pancreas. Fractionalislet blood flow was expressed as a percentage of whole pancreaticbloodflow.

Evaluation of the two-color microsphere method. Black and green E-Z microspheres were used in anesthetized rats (n = 8). The order of administration was switched every experiment.A nonmetabolizable glucose derivative, 3-O-methylglucose (5 g/kg;Sigma Chemical, St Louis, MO), was injected via the femoral vein8 min after the first microsphere injection and was followed 3min later by the second microsphereinjection.

Comparison of effect of hyperglycemia on islet perfusion in anesthetized and conscious rats. Islet blood flow in basal and glucose-stimulated states was measured using the two-color microsphere method in pentobarbital-anesthetized(n = 10) and conscious (n = 9) rats. Glucose solution (50%; 5g/kg) was injected via the carotid artery catheter 8 min afterthe first microsphere injection. The second microsphere injectionwas administered 3 min after the glucosesolution.

Effect of hypoglycemia on islet perfusion in conscious rats. Four units of regular human insulin (Novo, Bagsvaerd, Denmark) were administered via the carotid artery catheter after thefirst microsphere injection, and blood glucose was measured every10 min. Once the blood glucose level fell below 2.7 mmol/l, thesecond microsphere injection was administered. In a separate experiment,atropine methyl bromide (10 mg/kg; Sigma) was injected via thecarotid artery catheter 15 min before the first microsphere injectionto block peripheral parasympathetic, muscarinic receptors. Methylatropinedoes not readily cross the blood-brain barrier and thus does notimpair central nervous system muscarinic cholinergic neurotransmission.This dose of methylatropine did not significantly inhibit theincrease of plasma glucagon observed during insulin-induced hypoglycemia(7).

Statistical analysis. Values are expressed as means ± SE. Student's paired t-test was used for comparison of data from the same animal. Student'sunpaired t-test was used for comparison of two groups, and ANOVAand Scheffé's test as a post hoc test were used for comparisonof multiple groups. Differences were considered significant ifthe P value was <0.05.

	RESULTS

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The two-color-microsphere method was evaluated using two approaches: by comparison with NEN microspheres and by using thenonmetabolizable glucose analog 3-O-methylglucose, which is knownto have no effect on islet perfusion (Table 1) (12). Bloodglucose, serum IRI, and mean arterial blood pressure were similarirrespective of whether NEN microspheres or E-Z microspheres wereused for experiments. In addition, there were no significant differencesin whole pancreatic blood flow, islet blood flow corrected forpancreatic weight, or estimated islet weight, fractional isletblood flow, or duodenal blood flow. Blood glucose, serum IRI,and mean blood pressure remained unchanged after 3-O-methylglucoseinjection. Blood flow measurement with black and green E-Z microspheresrevealed that intravenous injection of 3-O-methylglucose had noeffect on whole pancreatic, islet, fractional, or duodenal bloodflows.

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Table 1. Evaluation of 2-color microsphere method in anesthetized rats

As shown in Table 2, both blood glucose and serum IRI increased in anesthetized and conscious rats after glucose injection.Blood glucose, however, was significantly higher, and serum IRIwas lower after a glucose load in pentobarbital-anesthetized ratsthan in conscious rats. Mean blood pressure did not differ significantlybetween anesthetized and conscious rats. Whole pancreatic bloodflow significantly increased in both groups after glucose injection,and there were no significant differences between the two groups.Islet blood flow increased in anesthetized rats by 111% and inconscious rats by 150%. No differences were observed in isletblood flow corrected for pancreatic or islet weight between anesthetizedand conscious rats. In the basal state, fractional islet bloodflow was significantly higher in anesthetized rats than in consciousrats. This parameter rose in both groups after glucose injection,but it did not differ significantly between them. Duodenal bloodflow was significantly reduced in anesthetized rats compared withconscious rats in the basal state, whereas it did not differ afterglucose injection.

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Table 2. Basal and glucose-stimulated islet blood flow in anesthetized and unanesthetized rats

After insulin administration to conscious rats (Table 3), blood glucose was reduced, but blood pressure remained unchanged.Whole pancreatic blood flow and duodenal blood flow were significantlyincreased during hypoglycemia. However, islet blood flow correctedfor pancreatic or islet weight was not affected by insulin-inducedhypoglycemia, whereas fractional islet blood flow was significantlydecreased. Methylatropine pretreatment did not significantly alterblood glucose or blood pressure. However, basal pancreatic andislet blood flows were significantly reduced by pretreatment withmethylatropine. During hypoglycemia, however, whole pancreaticand islet blood flows were significantly increased in methylatropine-treatedrats by 239% and 181%, respectively. Islet blood flow was significantlyelevated compared with that without methylatropine pretreatment.No significant changes were observed in fractional islet or duodenalblood flow during hypoglycemia after methylatropine pretreatment.

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Table 3. Effect of insulin-induced hypoglycemia on islet blood flow in unanesthetized rats

	DISCUSSION

TOP ABSTRACT INTRODUCTION METHODS RESULTS DISCUSSION REFERENCES

E-Z microspheres are commercially available in six different colors at present; however, only the combination of black andgreen microspheres was applicable to measurement of islet perfusionin our study. E-Z microspheres differ from NEN microspheres inthat they have a larger size variation and a density closer tothat of red blood cells. However, we demonstrated very similarislet blood flow with either NEN or E-Z microspheres. Jansson(10) reported that basal islet blood flow in rats was 40-70µl · min¹ · g pancreas¹ using NEN microspheres, a value about one-half that which weobtained in the experiments reported here. However, when isletblood flow was corrected for islet tissue weight, our result issimilar to that reported by Jansson's group, 6.1 ml · min¹ · g islet tissue weight¹ in anesthetized normal Wistar rats (5). This indicates thatislet blood flow is more appropriately expressed as correctedfor islet tissue weight. The comparison of NEN and E-Z microspheresand the lack of effects of 3-O-methylglucose on islet blood flowvalidated the two-color microsphere method for measurement ofislet perfusion inrats.

Pentobarbital sodium has suppressant actions on the cardiovascular system with reduction in cardiac output, depression ofsympathetic and parasympathetic functions, and lowering of bloodpressure in rats (19). Conversely, surgical stresses such asneck surgery and catheter implantation activate the sympatheticnervous system and offset the hypotensive effects of pentobarbitalsodium. Hindlycke and Jansson (9) investigated the effectsof various anesthetic agents on islet perfusion. They found thatislet blood flow was increased by chloral hydrate but markedlydecreased by ketamine and xylazine compared with pentobarbitalor thiobutabarbital anesthesia. We demonstrated that islet bloodflow was not affected by pentobarbital anesthesia compared withconscious rats. This result was somewhat unexpected, because pancreaticislets are richly innervated (1) and islet perfusion is regulatedby a neural mechanism (10, 13). Previous studies have shownthat nitric oxide synthase inhibitors caused a marked reductionin islet perfusion (16, 21), suggesting that nitric oxidereleased from endothelial cells may locally regulate islet bloodflow. The finding that anesthesia and surgical stress did notaffect islet perfusion indicated that local regulation of isletperfusion might be more predominant than neural regulation duringhyperglycemia.

Hypoglycemia induces systemic hemodynamic changes including increased cardiac output; increased blood flow to brain, skeletalmuscle, and foregut; and decreased blood flow to kidneys and spleen(8). With regard to the splanchnic circulation, blood flowin the superior mesenteric artery increased by 53% in healthysubjects during hypoglycemia, as demonstrated using a Dopplertechnique (2). This may result in an increased metabolic fuelsupply for hepatic gluconeogenesis via the portal system. Thisis consistent with increased blood flow documented in the wholepancreas and duodenum during hypoglycemia in the present study.Sparrow and Beckingham (20) reported that hypoglycemia increasedpancreatic islet blood flow by 221% in pentobarbital-anesthetizedrats, whereas whole pancreatic blood flow remained unchanged.They suggested that the increase in islet perfusion might be explainedby increased activity of islet $alpha$ -cells to secrete glucagon duringhypoglycemia, although $alpha$ -cells constitute only a minor proportionof islet cells as a mantle. In contrast to this, our results demonstratedthat islet perfusion remained unchanged, whereas whole pancreaticblood flow was increased and fractional islet blood flow was decreasedduring hypoglycemia. This discrepancy with the previous resultsmay be due to the anesthesia used in the previous study. Becausethe remaining $beta$ -cells are suppressed to decrease endogenous insulinsecretion during hypoglycemia, this is compatible with the unchangedislet blood flow and decreased fractional islet blood flow observedin ourstudy.

The vagus nerve participates in the regulation of whole pancreatic and islet perfusion (10). In the present study, wholepancreatic and islet blood flow decreased by peripheral blockadeof parasympathetic nerves with methylatropine. Atropine directlysuppresses pancreatic exocrine and endocrine secretion in thenonfasting state (1, 18), which may be associated with thereduced whole pancreatic and islet blood flow. In previous studies,however, basal whole pancreatic and islet perfusion were not affectedby atropine administration or vagotomy in anesthetized rats (13).This discrepancy may also be explained by the use of anestheticagents. Because hypoglycemia strongly stimulates the autonomicnervous system, peripheral cholinergic muscarinic blockade manifestsas adrenergic activation. In general, vagal cholinergic nervesstimulate islet blood flow, whereas adrenergic effects on isletperfusion are complex (10). Norepinephrine infusion and $beta$ ₂-adrenoceptorstimulation induced a decrease in islet blood flow, and $alpha$ -receptorstimulation and isoproterenol infusion induced an increase inislet perfusion (11, 15, 17). The finding that pretreatmentwith methylatropine increased islet perfusion during hypoglycemiais in marked contrast to the finding that atropine or vagotomyabolished a glucose-stimulated increase in islet perfusion (13).However, the effect of vagal muscarinic blockade was specificto islet blood flow in the latter but not in the former. The vagalnervous system is known to mediate the hyperglycemia-induced increasein islet blood flow (13). Therefore, it is interesting thatthe vagal nervous system also apparently prevents an increasein islet perfusion duringhypoglycemia.

In conclusion, we developed a two-color microsphere technique in conscious rats. Basal and glucose-stimulated islet bloodflow levels were similar in pentobarbital-anesthetized and consciousrats. However, the basal distribution of blood flow within thepancreas was altered by anesthesia. Insulin-induced hypoglycemiaincreased whole pancreatic blood flow, whereas it failed to changeislet blood flow, and blood flow diversion to pancreatic isletswas decreased in conscious rats. Because pretreatment with methylatropineincreased islet blood flow during hypoglycemia, prevention ofthis increase in islet perfusion during hypoglycemia may be mediated,at least in part, by a cholinergic, vagal muscarinicmechanism.

Perspectives

Pancreatic islet blood flow may be measured in the conscious state using colored microspheres at two time points. The lackof effect of anesthesia on a glucose-induced increase in isletperfusion suggests that this phenomenon may be essential in responseto acute hyperglycemia. Islet blood flow appears to be regulatedaccording to the activity of pancreatic islets during hyperglycemiaor hypoglycemia in a manner independent of the exocrine pancreas.This once again emphasizes the importance of regulation of pancreaticislet perfusion in isletfunctions.

	ACKNOWLEDGEMENTS

The authors are grateful to K. Sekioka and J. Ishimatsu for technicalassistance.

	FOOTNOTES

This work was supported in part by the Ministry of Education, Science, Sports and Culture grant-in-Aid for Science Research(C) (11671128),1999.

Address for reprint requests and other correspondence: M. Iwase, Dept. of Medicine and Clinical Science, Graduate School ofMedical Sciences, Kyushu Univ., Maidashi 3-1-1, Higashi-ku, Fukuoka812-8582, Japan (E-mail: iwase{at}intmed2.med.kyushu-u.ac.jp).

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.Section 1734 solely to indicate thisfact.

Received 3 May 2000; accepted in final form 8 January 2001.

	REFERENCES

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