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The hyperinsulinemic-euglycemic clamp is the "gold standard" for the assessment of insulin action. Insulin is infused at a constant rate stimulating glucose uptake. The amount of exogenous glucose infused to counter this drop is indicative of insulin sensitivity. Here the procedure is performed on a conscious, unrestrained rat.
Type 2 diabetes (T2D) is rapidly rising in prevalence. Characterized by either inadequate insulin production or the inability to utilize insulin produced, T2D results in elevated blood glucose levels. The "gold-standard" in assessing insulin sensitivity is a hyperinsulinemic-euglycemic clamp or insulin clamp. In this procedure, insulin is infused at a constant rate resulting in a drop in blood glucose. To maintain blood glucose at a constant level, exogenous glucose (D50) is infused into the venous circulation. The amount of glucose infused to maintain homeostasis is indicative of insulin sensitivity. Here, we show the basic clamp procedure in the chronically catheterized, unrestrained, conscious rat. This model allows blood to be collected with minimal stress to the animal. Following the induction of anesthesia, a midline incision is made and the left common carotid artery and right jugular vein are catheterized. Inserted catheters are flushed with heparinized saline, then exteriorized and secured. Animals are allowed to recover for 4-5 days prior to experiments, with weight gain monitored daily. Only those animals who regain weight to pre-surgery levels are used for experiments. On the day of the experiment, rats are fasted and connected to pumps containing insulin and D50. Baseline glucose is assessed from the arterial line and used a benchmark throughout the experiment (euglycemia). Following this, insulin is infused at a constant rate into the venous circulation. To match the drop in blood glucose, D50 is infused. If the rate of D50 infusion is greater than the rate of uptake, a rise in glucose will occur. Similarly, if the rate is insufficient to match whole body glucose uptake, a drop will occur. Titration of glucose continues until stable glucose readings are achieved. Glucose levels and glucose infusion rates during this stable period are recorded and reported. Results provide an index of whole body insulin sensitivity. The technique can be refined to meet specific experimental requirements. It is further enhanced by the use of radioactive tracers that can determine tissue specific insulin-stimulated glucose uptake as well as whole body glucose turnover.
A: Surgical Catheterization of Arterial and Venous Circulation
Part 1: Arterial and Venous Catheter Preparation
Part 2: Surgical Preparation
Part 3: Surgery
B: Postoperative Care
Part 1: Immediate Postoperative Care and Monitoring
Part 2: Maintaining Catheter Patency
C: Hyperinsulinemic-Euglycemic Clamp
Part 1: Clamp Set-up and Preparation
Part 2: Experimental Protocol
D: Hyperinsulinemic-Euglycemic (Insulin) Clamp Results
When performed correctly, the clamp procedure assesses the steady state insulin sensitivity of the rat. In presenting data obtained from the clamp, it is essential to document glucose levels and glucose infusion rates. Stable glucose levels over a time course of a minimum of 30min (Figure 3) are indicative of a steady state. Glucose is considered stable only if whole blood glucose is maintained within ~1mM. Glucose infusion rates show the levels of exogenous glucose required to maintain glycemia. Where possible, these figures should be shown as a time course rather than single, averaged value (Figure 4).
Other recommended measures to be reported are plasma insulin and hematocrit. The determination of both fasting and clamped insulin levels confirm that insulin has been successfully administered and will detect any differences in levels between treatment groups (Figure 5). Obtaining hematocrit measures at baseline and at the conclusion of the insulin clamp are suggested (Figure 6). This is to ensure hematocrit levels do not fall more than 5% during the experiment and the accompanying alterations in blood volume and flow do not influence glucose disposal.
Figure 1. Experimental set-up. Figure 1 shows unrestrained, conscious rat during the clamp procedure. Catheters allow blood sampling and infusions without handling the animal. Pumps to the left contain insulin and glucose.
Figure 2. Expected data during the clamp procedure. To obtain a clamp at baseline levels (euglycemia, 5mM), the levels of exogenous glucose (D50) are manipulated until the baseline or 'clamp' is achieved.
Figure 3. Expected plasma glucose results of the clamp procedure. When the animal is 'clamped', blood glucose is relatively stable across time and experimental groups.
Figure 4. Representative glucose infusion rates of the clamp procedure. The amount of exogenous glucose required to maintain euglycemia differs. This is illustrated with a control (chow fed) and high fat fed (insulin resistant) animals. The high fat fed animal requires less glucose infused to maintain glycemia, primarily because it is insensitive to the insulin infused.
Figure 5. Representative plasma insulin of the rat. The plasma insulin during the insulin clamp should be higher than the fasted, baseline plasma insulin. This ensures insulin was properly administered to the animal during the insulin clamp.
Figure 6. Reporting hematocrit. The baseline hematocrit and hematocrit following the experiment must be obtained and reported. This ensures hematocrit levels do not fall more than 5% of baseline levels resulting from excessive arterial blood sampling.
Initially developed for investigation of insulin sensitivity in humans, the clamp procedure has now been adapted to other species including laboratory rats and mice. Investigating animal models of insulin resistance provides a significant aid in understanding the pathophysiology of insulin sensitivity and associated pathologies as well as identifying therapeutic interventions that have clinical value1,2. Several methods to evaluate insulin sensitivity in animals have been employed3. Such techniques ...
Procedures were approved by the University of Calgary Animal Care and Use Committee and abide by the Canadian Association for Laboratory Animal Science guidelines for experimentation. The authors have no conflicting interests or disclosures.
This study was supported by the Canadian Institutes of Health Research and Genome Canada.JS holds salary support awards from the Alberta Heritage Foundationfor Medical Research, Heart and Stroke Foundation of Canadaand the Canadian Diabetes Association. Special thanks to Dr. David Wasserman and Bingle Bracy for teaching this procedure to the Shearer laboratory.
Name | Company | Catalog Number | Comments |
Name of the reagent | Company | Catalogue number | Comments (optional) |
Intramedic Polyethylene Tubing (PE-50) | Fisher Scientific | 14-170-12B | Internal diameter of .58mm (.023") x Outer diameter of .965mm (.038") |
Dow Corning Silastic Laboratory Tubing | Fisher Scientific | 11-189-15C | Internal diameter of .76mm (0.030") x Outer diameter of 1.65mm (0.065") |
Tygon S-50-HL Medical Tubing | Harvard Apparatus | PY2 72-1251 | Internal diameter of 3.2mm (0.125") x Outer diameter of 4.7mm (0.1875") |
Loctite Super Glue | Grand & Toy | 32237 | Gel Control |
Sterile Surgical Blade | VWR | BD371610 | |
Curved Micro Dissecting Forceps | George Tiemann & Co. | 160-20 | x 2 |
Straight Micro Dissecting Forceps | George Tiemann & Co. | 160-15 | x 2 |
Curved Hemostat | George Tiemann & Co. | 105-1135 | x 2 |
Straight Hemostat | George Tiemann & Co. | 105-1130 | x 2 |
Hemostat Tip Guards | Robbins Instruments, Inc. | 15.09-2-004 | |
Straight Surgery Scissors | George Tiemann & Co. | 105-402 | |
VENOJECT Multi-Sample Luer Adapter | Terumo Medical Products | 810127A | 21 guage, 1 in. |
Sterile Catheter Introducer | Becton Dickinson | 406999 | |
14-gauge Blunt Needle | Becton Dickinson | 511310 | 14 guage, 2 in. |
Sterile Surgical Suture | Johnson & Johnson Medical Products | 1679H | Silk, size 3-0 |
Non-Sterile Surgical Suture | Angiotech Pharmaceuticals, Inc. | SP116 | Silk, size 4-0 |
Cotton Swabs | VWR | 10806-005 | |
4ply Gauze Pads | VWR | CA43845-062 | |
Small Animal Cordless Clippers | Harvard Apparatus | 729063 | |
Isoflurane | Halocarbon Products Corp. | IPN-45 | |
Anesthetic Cart | Benson Medical Industries, Inc. | ||
70 % Ethanol | Fisher Scientific | HC-1000 | |
Betadine Antiseptic Solution | Western Drug Distribution Centre Ltd. | 105267 | |
Model 11 Plus Syringe Pump | Harvard Apparatus | 702208 | |
Stainless Steel Tubing Couplers | Harvard Apparatus | 72-4434 | 23 gauge, 0.3 in. |
Stainless Steel Tubing Plugs | Harvard Apparatus | 72-4436 | 23 gauge, 0.5 in. |
Stainless Steel Blunt Needles | Instech Laboratories, Inc. | LS22 | 22 gauge |
60 Degree Y-Connectors | Small Parts | STCY-22-05 | 22 gauge |
CritSpin Micro-hematocrit Centrifuge | Iris Sample Processing | CS12 | |
Mini Centrifuge | Fisher Scientific | 05-090-100 | |
Micro Centrifuge Tubes | VWR | 53550-778 | |
50ml polypropylene centrifuge tubes | VWR | 89004-364 | |
1ml Plastic Slip Tip Syringes | Becton Dickinson | 309602 | |
3ml Plastic Luerlok Tip Syringes | Becton Dickinson | 309585 | |
Heparin Anticoagulant Injection | Western Drug Distribution Centre Ltd. | 102824 | Manufacturer: LEO Pharma Inc. Conc. 1000 IU |
EDTA Solution | Promega Corp. | V4231 | 0.5 M, pH 8.0 |
Saline | Western Drug Distribution Centre Ltd. | ABB7983154 | Manufacturer: Hospira 0.9% Sodium Chloride |
50% Dextrose | Vetoquinol | 8DEX012D | |
Humulin-R | Eli Lilly | HI-210 | 100U/ml |
1ml Insulin Syringes | Becton Dickinson | 309311 | |
Fisherbrand* Hemato-Seal Sealant | Fisher Scientific | 02-678 | |
Fisherbrand* Microhematocrit Capillary Tubes | Fisher Scientific | 22-362-574 | |
One Touch Ultra Test Strips | LifeScan, Inc. | AW 085-314H | |
One Touch Ultra Blood Glucose Meter | LifeScan, Inc. | AW 085-314B | |
Sodium Pentobarbitol | Ceva Sante Animale | 1715 138 | Conc. 54.7mg/ml |
Red Laboratory Labeling Tape | VWR | 89097-932 | |
Blue Laboratory Labeling Tape | VWR | 89097-936 | |
Weigh Scale | Fisher Scientific | 01-913-88 | |
Vortex | VWR | 58815-234 | |
Timer | VWR | 62344-641 |
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