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Effects of two commercially available feline diets on glucose and insulin concentrations, insulin sensitivity and energetic efficiency of weight gain

Published online by Cambridge University Press:  12 October 2011

M. Coradini*
Affiliation:
Centre for Companion Animal Health, School of Veterinary Science, The University of Queensland, Saint Lucia, Brisbane, QLD 4072, Australia
J. S. Rand
Affiliation:
Centre for Companion Animal Health, School of Veterinary Science, The University of Queensland, Saint Lucia, Brisbane, QLD 4072, Australia
J. M. Morton
Affiliation:
Centre for Companion Animal Health, School of Veterinary Science, The University of Queensland, Saint Lucia, Brisbane, QLD 4072, Australia
J. M. Rawlings
Affiliation:
WALTHAM Centre for Pet Nutrition, Melton Mowbray, Leicestershire LE14 4RT, UK
*
*Corresponding author: M. Coradini, fax +61 7 3346 9822, email [email protected]
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Abstract

A low-carbohydrate, high-protein (LCHP) diet is often recommended for the prevention and management of diabetes in cats; however, the effect of macronutrient composition on insulin sensitivity and energetic efficiency for weight gain is not known. The present study compared the effect in adult cats (n 32) of feeding a LCHP (23 and 47 % metabolisable energy (ME)) and a high-carbohydrate, low-protein (HCLP) diet (51 and 21 % ME) on fasting and postprandial glucose and insulin concentrations, and on insulin sensitivity. Tests were done in the 4th week of maintenance feeding and after 8 weeks of ad libitum feeding, when weight gain and energetic efficiency of each diet were also measured. When fed at maintenance energy, the HCLP diet resulted in higher postprandial glucose and insulin concentrations. When fed ad libitum, the LCHP diet resulted in greater weight gain (P < 0·01), and was associated with higher energetic efficiency. Overweight cats eating the LCHP diet had similar postprandial glucose concentrations to lean cats eating the HCLP diet. Insulin sensitivity was not different between the diets when cats were lean or overweight, but glucose effectiveness was higher after weight gain in cats fed the HCLP diet. According to the present results, LCHP diets fed at maintenance requirements might benefit cats with multiple risk factors for developing diabetes. However, ad libitum feeding of LCHP diets is not recommended as they have higher energetic efficiency and result in greater weight gain.

Type
Full Papers
Copyright
Copyright © The Authors 2011

There are currently a large number of diets available commercially for cats, which vary greatly in nutrient composition. Cats are strict carnivores and do not metabolise carbohydrates efficiently(Reference Kienzle1Reference Kienzle5). The typical prey diet of cats is low in carbohydrate ( < 10 % metabolisable energy (ME))(Reference Eisert6); however, most commercially available dry cat foods are moderate to high in carbohydrate content (>25–55 % ME), partly because of the difficulty in formulating extruded, dry diets that are low in carbohydrate, and partly because cereal is a relatively inexpensive ingredient, and there is demand for lower-cost diets in the pet food market.

Low-carbohydrate, high-protein (LCHP) diets have been reported in research abstracts and in a recent publication to significantly reduce the postprandial increase in blood glucose concentration compared with high-carbohydrate, low-protein (HCLP) diets (Farrow HA, Rand JS and Sunvold GD (2002); Singh R, Rand J and Morton J (2006), unpublished results)(Reference Hewson-Hughes, Gilham and Upton7), possibly indicating a reduced demand on the β-cells to produce insulin. A LCHP diet has also been shown to reduce the need for exogenous insulin administration in diabetic cats(Reference Bennett, Greco and Peterson8). Diabetes in cats is similar to human type 2 diabetes, characterised by decreased insulin secretion and insulin resistance(Reference Rand9, Reference Stumvoll, Goldstein and Van Haeften10), and it has been hypothesised that a high-carbohydrate diet fed long term potentially might be a risk factor for the development of diabetes mellitus in cats(Reference Rand, Fleeman and Farrow11).

Increased body fat mass in cats is associated with decreased insulin sensitivity and hyperinsulinaemia, and is a known risk factor for feline diabetes(Reference Scarlett and Donoghue12, Reference Appleton, Rand and Sunvold13). In neutered cats, weight gain is positively correlated with the percentage of dietary fat(Reference Backus, Cave and Keisler14). Both hyperglycaemia and insulin resistance increase the demand on the pancreatic β-cells to produce insulin to maintain glucose homeostasis, ultimately predisposing to β-cell failure and overt diabetes(Reference Porte15). As in humans, healthy cats demonstrate a range of underlying insulin sensitivities(Reference Appleton, Rand and Sunvold13). Cats with insulin sensitivities below a study population median were found to be at increased risk of developing impaired glucose tolerance with obesity, and presumably with sufficient time, or imposition of another risk factor such as steroid administration, were at increased risk of developing type 2 diabetes(Reference Appleton, Rand and Sunvold13).

The effect of dietary macronutrient composition on fasting and postprandial plasma glucose and insulin concentrations over 24 h after eating has been inadequately investigated in cats, and it is not known how diet might affect insulin sensitivity and energetic efficiency for weight gain.

It was hypothesised that compared with a LCHP diet, feeding a HCLP diet to cats results in higher postprandial glucose and insulin concentrations, and is associated with lower insulin sensitivity, but may result in lower weight gain when fed ad libitum.

The aims of the present study were to compare the effect of feeding two commercially available diets, LCHP and HCLP diet, first, in ideal weight, clinically healthy cats and, second, after 8 weeks of ad libitum feeding to promote weight gain. Specific variables of interest were dietary effects on insulin sensitivity, fasting and postprandial plasma glucose and insulin concentrations before and after weight gain, and energetic efficiency of weight gain.

Materials and methods

Animals

A total of thirty-two neutered, lean, mixed breed cats (sixteen males, sixteen females) were used in the study. Accurate ages were unknown, but estimated to be from 2–4 years based on visual and physical examination, including examination of dentition. Cats were sourced from a municipal pound and all were rehomed at the end of the study.

Cats were considered healthy based on clinical examination, haematological and serum biochemical profiles, and a negative feline immunodeficiency virus test (Agen Biomedical Limited, Brisbane, QLD, Australia). Mean body condition score was 4·9 (range 4–5) on a nine-point body condition system(Reference Laflamme16). Mean body weight was 3·31 (sd 0·82) kg. The study protocol, care and handling of the animals were approved by the University of Queensland's Animal Ethics Committee under the Animal Welfare Act of the State of Queensland and the WALTHAM Ethical Review Committee (approval no. SVS/328/06/ARC). Cats were housed in environmentally enriched rooms for 12 weeks before and during the study. At 4 weeks before the beginning of the study, cats were individually housed and allowed at least 4 h of socialisation and exercise daily.

Experimental design

Dietary treatments

The present study used commercially available, extruded, dry diets that complied with the Association of American Feed Control Officials standards for complete and balanced feline diets. The following three diets were used in the study: diet 1 was a ‘washout’ or baseline diet, moderate in carbohydrate, fat and protein; diet 2 was a LCHP diet; diet 3 was a HCLP diet. A list of ingredients used in each diet is shown in Table 1. Dietary analysis was performed by an independent laboratory (DTS Food Laboratories, Kensington, VIC, Australia) accredited by the National Association of Testing Authorities. Digestibility trials were performed according to the Association of American Feed Control Officials' guidelines by the manufacturers (diets 1 and 3: Mars Petcare, Raglan, NSW, Australia; diet 2: Royal Canin, Aimargues, France), and involved six adult cats fed at maintenance energy requirements. The study consisted of three phases (Table 2).

Table 1 Diet analyses, main ingredients, digestibility and energetic density of each diet

LCHP, low carbohydrate, high protein; HCLP, high carbohydrate, low protein; NFE, nitrogen-free extract; ME, metabolisable energy; NRC, National Research Council.

* Whiskas Adult with Vita-Bites, Mars Petcare (Raglan, NSW, Australia).

Royal Canin Diabetic Feline, Royal Canin (Aimargues, France).

Kitekat Krunch, Mars Petcare.

§ NFE = 100 − (moisture+protein+fat+crude fibre+ash).

Included vitamins A, D3, E, thiamin, riboflavin, pantothenic acid, niacin, pyridoxine, folic acid, cyanocobalamin, choline and biotin. Vitamin C was included in the LCHP diet.

Included Ca, P, K, Na, Cl, Mg, and trace elements Fe, Cu, Mn, Zn, I and Se.

** Apparent percentage of DM digestibility = (food ingested (g) − faeces produced (g)) × 100/food ingested (g), calculated on a DM basis.

†† Calculated using the equation proposed by the NRC(50).

‡‡ Calculated using the modified Atwater factors(51).

Table 2 Timeline of feeding and test weeks

B, baseline; LCHP, low carbohydrate, high protein; M, maintenance; HCLP, high carbohydrate, low protein.

* In the third test week (week 17), cats were fed a restricted amount of food to maintain their weights measured on week 16 within 95–105 %.

Dual-energy X-ray absorptiometry scans were performed in fifteen cats.

In the baseline phase, all cats were fed the baseline or ‘washout’ diet for 4 weeks, which was moderate in carbohydrate and protein (Table 1), and energy intake was restricted to maintain the cats’ body weight within 95–105 % of their initial weight. Baseline testing was conducted in the 4th week of feeding (Table 2). In the second week of feeding the baseline diet, food was withheld for 24 h, and a 2 ml fasting blood sample was collected from the jugular vein, to determine each cat's insulin sensitivity status based on the simple measure of insulin sensitivity, the fasting glucose:insulin ratio(Reference Appleton, Rand and Sunvold17). Cats were then paired based on sex, insulin sensitivity and body weight. Immediately after the baseline testing in the 4th week, cats within each pair were randomly allocated to receive either the LCHP diet or the HCLP diet (Table 1). Random allocation was done by drawing numbers corresponding to each cat; the first cat of the pair drawn was allocated the LCHP diet, and its pair was automatically assigned the HCLP diet.

During the second phase or stable-weight phase (weeks 5–8), cats were fed for 4 weeks their respective diets to maintain body weight within 95–105 % of their initial weight. Tests to compare the two test diets were performed in the 4th week of feeding (8th week of the study; Table 2).

In the third phase or the weight-gain phase (weeks 9–16), cats were fed their respective diets ad libitum for 8 weeks. In the 9th week (17th week of the study), cats were fed maintenance energetic requirements, and tests were performed to compare the two diets (Table 2).

Food intake was recorded daily and cats were weighed weekly for the duration of the study.

Testing protocol

General sampling methods

On day 1 of each test week, cats were anaesthetised with alfaxalone (Alfaxan-CD RTU; Jurox Private Limited, Rutherford, NSW, Australia), and a jugular catheter (Arrow International, Reading, PA, USA) was placed percutaneously for blood sampling. Catheter patency was maintained by flushing with a heparinised (Heparin Injection BP; Mayne Pharma Private Limited, Melbourne, VIC, Australia) saline solution (20 IU heparin/ml of 0·9 % saline solution) twice daily. This was followed by a dual-energy X-ray absorptiometry scan on day 3, an insulin-modified intravenous glucose tolerance test on day 5 and a 24 h meal-feeding test on day 7. Before each test, cats had food withheld for 24 h. They were fed immediately after each test was concluded. Packed cell volume was monitored, and there were no significant differences before and after each metabolic test, or between tests (data not shown).

Dual-energy X-ray absorptiometry scans

Total and abdominal fat and lean body masses were measured by dual-energy X-ray absorptiometry with a fan-beam X-ray bone densitometer, using a small animal protocol (Lunar Prodigy, enCORE GE Lunar software platform, version 9.10.108; GE Lunar Incorporation, Madison, WI, USA). Cats were anaesthetised with alfaxalone intravenously, to effect. Whole-body scans were done with cats placed in ventrodorsal recumbency.

Insulin-modified frequently sampled intravenous glucose tolerance test with minimal model analysis

Before sampling, 2 ml of blood were removed to clear the catheter of saline-diluted blood. After each sample collection, the saline-diluted blood was re-injected and the catheter flushed with 1 ml of saline solution and 1 ml of heparinised saline solution (5 IU heparin/ml of 0·9 % saline solution). The latter was done only when there were 2 min or more between sample collections.

The test was conducted as described previously(Reference Welch, Gebhart and Bergman18), except that the sample collected at 20 min in that study was collected at 19 min in the present study. Briefly, four baseline blood samples were collected before a glucose (Glucose Injection BP 50 %; Astra Zeneca Proprietary Limited, Sydney, NSW, Australia) bolus of 0·3 g/kg was administered intravenously, and twenty-nine blood samples were collected in the subsequent 3 h. At 20 min, 0·05 IU regular human insulin/kg (Humulin R; Eli Lilly, Sydney, Australia) were injected as a bolus, intravenously. The computer program Minimal Model Millennium (MinMod Millennium, version 6.02; MINMOD Inc., 2001, Los Angeles, CA, USA) was used to determine the insulin sensitivity index and glucose effectiveness based on values obtained from plasma glucose and insulin concentrations at each time point(Reference Boston, Stefanovski and Moate19).

Meal-feeding test

Before sampling, 2 ml of blood were removed to clear the catheter of saline-diluted blood. After each sample collection, the saline-diluted blood was re-injected and the catheter flushed with 1 ml of saline solution and 1 ml of heparinised saline solution (5 IU heparin/ml of 0·9 % saline solution or 10 IU heparin/ml of 0·9 % saline solution when there were 6 h between blood sampling).

At 30 and 5 min before the meal, two fasting blood samples were collected. At time 0, a meal consisting of 167 kJ/kg was fed, and at least 90 % consumed within 30 min. Then, eleven blood samples were collected in the subsequent 24 h, at 1, 2, 3, 4, 6, 8, 10, 12, 15, 18 and 24 h after the meal was offered. Immediately after collection, blood samples for glucose and insulin analyses were placed into sterile tubes containing EDTA and the proteinase inhibitor aprotinin (Trasylol; Bayer Limited, Sydney, NSW, Australia) at 0·05 ml/ml of blood collected. Samples were kept on ice for 10–20 min until centrifuged for 8 min at 1500 g. After centrifugation, plasma was removed and stored in vials at − 70°C until analysis.

Erythrocyte auto-transfusion was performed during this test, to maintain erythrocyte mass as described previously(Reference Appleton, Rand and Priest20). In summary, after plasma was collected, erythrocytes remaining in the EDTA tubes were washed with 0·9 % saline, then resuspended in saline to the initial volume of blood taken and auto-transfused.

Sample analyses

Plasma glucose was determined using an enzymatic method (Hexokinase enzymatic UV; Olympus Diagnostic Systems Division, Melville, NY, USA), with mean intra-assay variability of 0·7 %, at glucose concentration of 3·3 mmol/l, and 0·5 % at glucose concentrations of 6·3 and 10·4 mmol/l. Mean inter-assay variability was 1·3, 1·0 and 1·1 %, respectively. Plasma insulin concentrations were determined by a commercially available RIA kit (Porcine Insulin RIA Kit; Linco Research, Inc., St Charles, MO, USA). The assay has 100 % specificity for human insulin, and was validated for the detection of feline insulin. Assay analytical sensitivity was 12·0 pmol/l. Inter-assay variation was 6·0 and 8·0 % at insulin concentrations of 44·9 and 204·5 pmol/l, respectively. Intra-assay variation was 6·5 %. Specificity was determined by dilutional parallelism. The standard curves remained parallel to a dilution of 40·0 %.

Calculations

For the 24 h meal-feeding test, fasting concentrations of glucose and insulin were estimated as the average of concentrations at − 30 and − 5 min. Time from the onset of feeding to (1) the time to glucose and insulin concentration first exceed fasting concentration, (2) time to peak concentration and (3) time to return to fasting concentration was calculated based on 90 % ranges of differences using the methodology as described previously(Reference Marshall, Rand and Morton21). For plasma glucose concentration, 90 % ranges of differences were 0·4 and 0·3 mmol/l, and those for plasma insulin concentration were 13·2 and 10·2 pmol/l in the second and third test weeks, respectively. Absolute values were used in the calculation of the 90 % ranges of difference for plasma glucose concentration, and ratios of means were used for plasma insulin concentration.

The postprandial period for glucose and insulin was defined as the time from when concentrations first exceeded fasting to the time to return to fasting concentrations.

Peak concentration was defined as the highest concentration observed after feeding, and was defined only for cats that exceeded fasting concentrations as described above.

Mean analyte concentration for 24 h was calculated as 24 h area under the curve using the trapezoidal method(Reference Rowland and Tozer22), and then divided by twenty-four.

Energetic efficiency of body-weight gain for the 8 weeks of ad libitum feeding was calculated for each cat as:

\begin{eqnarray} (Total energy intake for the 8 weeks of ad libitum feeding - sum of estimated daily energy requirements for the 8 weeks of ad libitum feeding)/body weight gained. \end{eqnarray}

Total energy intake and body weight gained were calculated from the 8 weeks of ad libitum feeding. Cats were generally weighed weekly. Linear interpolation between consecutive observed weights was used to estimate body weight on days when cats were not weighed. Each cat's daily energy requirement was then calculated for each day using the following formula(Reference Earle and Smith23, Reference Kienzle, Edtstadtler-Pietsch and Rudnick24):

\begin{eqnarray} Daily\,energy\,requirement = 151\cdot 8\times (body\,weight\,(kg))^{0\cdot 40} - 87\cdot 5. \end{eqnarray}

The constants of 151·8 and 87·5 were determined using daily energy requirements at the end of the 3rd week of maintenance feeding the baseline or ‘washout’ diet; body weight was the mean of each cat's daily weight during the 8 weeks of ad libitum feeding; the exponent of 0·40 was used because Earle & Smith(Reference Earle and Smith23) found that the daily energetic requirements/kg body weight decline with higher body weights. The exponent 0·4 removes the effect of weight differences on energy requirements of adult, intact and neutered colony cats(Reference Earle and Smith23). Energy efficiency estimates were used only for the twenty-eight cats that gained greater than 10 % body weight, as smaller weight gains would have been prone to greater measurement error, since an absolute error when measuring body weight equates to a much larger error when calculating energetic efficiency of body-weight gain if the actual body weight change is small.

Similarly, only cats that gained greater than 10 % body weight were used in the calculation of the percentage of weight gain that was accounted for by each of total and abdominal fat gain. The percentages of weight gain that was accounted for by each of total and abdominal fat gain were calculated as the change in total and abdominal fat masses, respectively, multiplied by 100 and divided by the change in weight from before to after weight gain.

Exclusions

In the stable-weight phase, one cat was excluded from the study in the second test week (week 8) because a catheter could not be placed in its jugular vein. Therefore, data from the stable-weight phase were analysed for fifteen of the sixteen cats enrolled in the LCHP group, and all sixteen cats enrolled in the HCLP group (Table 2).

During the weight-gain phase, one cat in the LCHP group was not blood sampled because a jugular catheter could not be inserted. Of the cats enrolled in the HCLP group, two were removed from the study at weeks 13 and 16 due to signs (diarrhoea) that indicated dietary intolerance. Data related to body weight, food and energy intake from these cats were included in statistical analyses, also data related to energetic efficiency of weight gain were included for the one of these two cats that had gained at least 10 % in body weight by the time it was removed from the study. During the third test week (week 17), dual-energy X-ray absorptiometry scans were performed in fifteen of the sixteen cats in the LCHP group and in fourteen of the sixteen cats in the HCLP group, and blood was collected from fourteen cats in each dietary group (Table 2).

Data from three cats fed the HCLP diet were not included in the calculation of energetic efficiency, because these cats gained less than 10 % in body weight during the ad libitum-feeding phase (refer to the section Materials and methods, Calculations).

Statistical analyses

Data were analysed using SigmaStat Version 3.0 (SPSS Incorporation, Chicago, IL, USA) and Stata Version 9.2 (StataCorp LP, College Station, TX, USA). The effects of diet on fasting, peak and mean concentrations of plasma glucose and insulin, on insulin sensitivity and glucose effectiveness were assessed using linear regression with pair fitted as a fixed effect. The individual cat was the unit of analysis. Mean glucose and insulin concentrations were compared between cats fed the LCHP and HCLP diets using linear regression. After inspection of distributions of dependent variables, all were log (base e)-transformed before analysis to better satisfy the assumptions behind linear regression. After such transformation, exponentiated β-coefficients for diet from the linear regression models can be interpreted as ratios of geometric means for the two diets.

Comparison between the amount of energy required to maintain body weight between the two test diets during the stable-weight phase was done using linear regression with diet and pair fitted as a fixed effect, without log transformation.

Food and energy intake, and energetic efficiency for weight gain were compared between the diets during the weight-gain phase using linear regression with pair fitted as a fixed effect without log transformation.

Times to first exceeding fasting concentration, times to peak concentration and times to return to fasting concentration for plasma glucose and insulin were compared between the dietary groups using log-rank tests for the equality of Kaplan–Meier survival functions. The individual cat was the unit of analysis. Times to return to fasting concentration were compared only using cats that had exceeding fasting concentration for the same analyte. Times to first exceeding fasting concentration were right-censored at 24 h for cats not exceeding fasting concentration; similarly, times to peak and to return to fasting concentration were right-censored at 24 h if peak concentration was not reached, or if concentration did not return to fasting, respectively. Distributions were also compared using Cox, Wilcoxon, Tarone–Ware and Peto-Peto-Prentice tests(Reference Hosmer, Lemeshow and May25). P values obtained were similar to those for the log-rank test, and are not reported.

Effects of weight gain on fasting, peak, and mean concentrations of plasma glucose and insulin were assessed by comparing these in cats at the end of the stable-weight phase (when cats were lean) with after the weight-gain phase (when cats were overweight) using linear regression with cat sampling as the unit of analysis, and with body weight status (lean or overweight), diet and cat fitted as fixed effects. Cat was fitted as a fixed effect to account for clustering of residuals due to the repeated measures within cat. Interactions between diet and body weight status were fitted and retained if appropriate. Data were log (base e)-transformed before analysis.

Body weight, lean and fat masses were compared between the ends of the stable-weight (week 8) and weight-gain phases (week 17) using linear regression with cat period as the unit of analysis, and with phase (stable-weight or weight-gain), diet and cat fitted as fixed effects, without log transformation. Interactions between diet and test phase were fitted and retained if appropriate.

Results

Baseline phase

For all variables measured, mean values were similar between the groups at the end of the baseline phase, after cats were fed for 4 weeks a moderate-carbohydrate baseline or ‘washout’ diet at maintenance energetic requirements (data not shown).

Body weight, fat and lean masses

During feeding at maintenance energy requirements (baseline and stable-weight phases), body weights did not vary by more than 5 % from initial body weight for any cat at any stage, and mean body weights were similar (3·4 and 3·2 kg) in the dietary groups at the end of the stable-weight phase (Table 3).

Table 3 Body weight, total and abdominal fat and lean masses measured at the beginning and at the end of the stable-weight phase, and at the end of the weight-gain phase, after 8 weeks of ad libitum feeding

(Mean values, percentages, standard deviations and 95 % confidence intervals)

LCHP, low carbohydrate, high protein; HCLP, high carbohydrate, low protein.

* Percentages calculated in relation to total body mass.

P value for interaction between lean/overweight and diet.

Estimate for the interaction term, i.e. estimated difference in change from lean to overweight between the diets.

§ n 16.

n 14.

After 8 weeks of ad libitum feeding, mean body weight increase was 37 (range 13–57) % with the LCHP diet and 17 (range − 0·8–36) % with the HCLP diet (Table 3). Increases for cats in the LCHP group were greater than for cats in the HCLP group; P values for interactions in body weight, total fat, abdominal fat and total lean mass between phase (end of stable-weight or end of weight-gain) and diet were < 0·01 (Table 3). Body condition scores were on average 6·3/9 for the LCHP group (range 5–7/9), and 5·8/9 for the HCLP group (range 5–7/9).

Of the weight gained in the LCHP group, total fat mass accounted for the majority (61 (sd 14·63)) %, of which more than one-quarter was abdominal fat (equating to 17 (sd 4·36) % of body weight gained). Similarly, most (55 (sd 12·62)) % of the weight gained in the HCLP group was due to total fat, of which more than one-quarter was abdominal fat (equating to 15 (sd 5·93) % of body weight gained; Table 3).

Effects of diet on plasma glucose concentration

Stable-weight phase

After eating the test diets fed to maintain body weight for 3 weeks, fasting glucose concentration did not differ significantly between the dietary groups (P = 0·29). However, peak concentration was 24 % or 1·5 mmol/l higher (P = 0·01) and mean concentration was 17 % or 0·9 mmol/l higher (P < 0·01) in cats fed the HCLP diet compared with those fed the LCHP diet (Table 4; Fig. 1(a)). Glucose concentration in two of the fifteen cats (13 %) in the LCHP group did not increase above fasting after the meal, and four of the sixteen cats (25 %) in the HCLP group had not returned to fasting concentration by the end of the meal-feeding test at 24 h (Table 5). The median times to exceed fasting, to peak and to return to fasting concentration did not differ significantly between the dietary groups (P ≥ 0·08; Table 5).

Table 4 Fasting, peak and mean concentrations of plasma glucose and insulin during a 24 h meal-feeding test, insulin sensitivity and glucose effectiveness based on the minimal model analysis of the insulin-modified intravenous glucose tolerance test at the end of the stable-weight phase, after lean cats had been fed a low carbohydrate, high protein or high carbohydrate, low protein diet maintaining their body weight for 3 weeks

(Mean values, standard deviations, ranges and 95 % confidence intervals)

LCHP, low carbohydrate, high protein; HCLP, high carbohydrate, low protein.

* Ratio of means (LCHP:HCLP), adjusted for pair.

Concentrations are reported as geometric means. Values have been reported only for cats from pairs in which both cats were tested; within each pair, one cat was allocated to each dietary group.

Excluding cats (n 13) whose concentrations did not increase significantly above fasting during the 24 h meal-feeding test.

Fig. 1 Comparison of the changes in plasma glucose concentration in the low carbohydrate, high protein (●) and high carbohydrate, low protein (○) dietary groups before and after weight gain. (a) End of stable-weight phase and (b) end of weight-gain phase. Values are means, with standard errors of the mean represented by vertical bars.

Table 5 Times (h) to exceed fasting concentration, times to peak and times to return to fasting concentration for plasma glucose and insulin during the 24 h meal-feeding test at the end of the stable-weight phase, after lean cats had been fed either the low carbohydrate, high protein or the high carbohydrate, low protein diet maintaining their body weight for 3 weeks

(25th percentiles, median values, 75th percentiles)

LCHP, low carbohydrate, high protein; HCLP, high carbohydrate, low protein.

* Calculated only for the thirteen cats in the LCHP group and the sixteen cats in the HCLP group whose concentrations increased significantly above fasting during the 24 h meal-feeding test.

Could not be calculated as not more than 75 % of cats had returned to fasting concentration by the end of observations at 24 h.

Weight-gain phase

After cats had been fed ad libitum for 8 weeks, mean fasting glucose concentration was 7 % or 0·4 mmol/l lower in cats fed the HCLP diet (P = 0·01), mean peak concentration was 27 % or 2·0 mmol/l higher (P = 0·01) and mean concentration over 24 h was 11 % or 0·64 mmol/l higher (P = 0·08) compared with cats fed the LCHP diet (Table 6; Fig. 1(b)). Whereas glucose had returned to fasting concentration by the end of the meal-feeding test in all cats in the HCLP group, in four of the fourteen cats (28 %) in the LCHP group, it was still significantly above fasting by the end of the 24 h test (Table 7). The increase in glucose concentration after eating occurred earlier in cats fed the HCLP diet than in cats fed the LCHP diet (P = 0·01; Table 7). Median times to peak and times to return to fasting concentration did not differ significantly between the dietary groups (P ≥ 0·74; Table 7).

Table 6 Fasting, peak and mean concentrations of plasma glucose and insulin during a 24 h meal-feeding test, insulin sensitivity and glucose effectiveness based on the minimal model analysis of the insulin-modified intravenous glucose tolerance test at the end of the weight-gain phase, after cats had been fed a low carbohydrate, high protein or high carbohydrate, low protein diet ad libitum for 8 weeks

(Mean values, standard deviations, ranges and 95 % confidence intervals)

LCHP, low carbohydrate, high protein; HCLP, high carbohydrate, low protein.

* Ratio of means (LCHP:HCLP), adjusted for pair.

Concentrations are reported as geometric means. Values have been reported only for cats from pairs in which both cats were tested; within each pair, one cat was allocated to each dietary group.

Table 7 Times to exceed fasting concentration, times to peak and times to return to fasting concentration for plasma glucose and insulin during the 24 h meal-feeding test at the end of the weight-gain phase, after cats had been fed the low carbohydrate, high protein or the high carbohydrate, low protein diet ad libitum for 8 weeks

(25th percentiles, median values, 75th percentiles)

LCHP, low carbohydrate, high protein; HCLP, high carbohydrate, low protein.

* Could not be calculated as not more than 75 % of cats had returned to fasting concentration by the end of observations at 24 h.

Effects of weight gain on plasma glucose concentration (comparison between the end of the stable-weight phase and the end of the weight-gain phase)

Compared with when cats were lean at the end of the stable-weight phase, 24 h mean glucose concentration increased significantly after a mean weight gain of 37 % in cats consuming the LCHP diet, but did not increase significantly after a mean weight gain of 17 % in cats fed the HCLP diet (Tables 4 and 6; Fig. 1(a) and (b)).

Compared with when cats were lean, after weight gain, mean fasting concentration was 0·1 mmol/l higher in cats fed the LCHP diet and 0·4 mmol/l lower in cats fed the HCLP diet. This change in fasting glucose concentration from when cats were lean to when they were overweight was NS for cats fed the LCHP diet (estimated change 2 %; 95 % CI − 4, 9 %; P = 0·44), but was significant after weight gain in cats fed the HCLP diet (estimated change 8 % lower; 95 % CI 2, 13 % lower; P = 0·01; significance of interaction P = 0·02). Peak glucose concentration was significantly higher after weight gain relative to when cats were lean in both dietary groups. Peak glucose increased by 1·2 mmol/l (estimated change 18 %; 95 % CI 10, 28 %; P < 0·01). There was no evidence of interaction between phase (end of stable-weight or end of weight-gain) and diet (P for interaction = 0·99). Compared with when cats were lean, mean glucose concentration was 11 % or 0·6 mmol/l higher after a mean weight gain of 37 % in cats fed the LCHP diet (95 % CI 5, 18 %; P < 0·01), but did not change significantly with a mean weight gain of 17 % in cats fed the HCLP diet (mean glucose concentration 0·2 mmol/l lower; estimated change 3 %; 95 % CI − 3, 9 %; P = 0·36). The P value for the interaction term was 0·05.

In lean cats fed the HCLP diet, mean plasma glucose concentration over 24 h did not differ significantly from cats fed the LCHP diet at the end of the weight-gain phase, which had gained an average of 37 % body weight (Fig. 1(a) and (b)). The estimated percentage difference between lean cats fed the HCLP diet relative to cats after weight gain in the ad libitum-feeding phase that were fed the LCHP diet was 5 % higher (95 % CI − 4, 16 %; P = 0·20).

Effects of diet on plasma insulin concentration

Stable-weight phase

Similar to glucose, fasting insulin concentration did not differ between the dietary groups after eating their respective diets, maintaining a lean body weight (P = 0·37). Peak concentration was 59 % or 64·1 pmol/l higher (P < 0·01) and mean concentration was 36 % or 24·7 pmol/l higher (P = 0·03) in cats fed the HCLP diet compared with cats fed the LCHP diet (Table 4; Fig. 2(a)). Plasma insulin concentration in two of the fifteen cats in the LCHP group (13 %) did not increase above fasting in the postprandial period (Tables 4 and 5).

Fig. 2 Comparison of the changes in plasma insulin concentration in the low carbohydrate, high protein (●) and high carbohydrate, low protein (○) dietary groups before and after weight gain. (a) End of stable-weight phase and (b) end of weight-gain phase. Values are means, with standard errors of the mean represented by vertical bars.

Weight-gain phase

After cats had been fed ad libitum for 8 weeks, fasting, peak and mean plasma insulin concentrations were not significantly different between the two dietary groups (P ≥ 0·12; Table 6; Fig. 2(b)). Similarly, the median times to exceed fasting, to peak and to return to fasting concentrations were not significantly different between the groups (P ≥ 0·30; Table 7; Fig. 2(b)).

Effects of weight gain on plasma insulin concentration (comparison between the end of the stable-weight phase and the end of the weight-gain phase)

In general, compared with when cats were lean at the end of the stable-weight phase, fasting, peak and mean insulin concentrations increased significantly after a mean weight gain of 37 % in cats consuming the LCHP diet, but did not increase significantly after a mean weight gain of 17 % in cats fed the HCLP diet (Tables 4 and 6; Fig. 2(a) and (b)).

Fasting insulin concentration increased 43 % or 13·8 pmol/l after weight gain in cats fed the LCHP diet (95 % CI 15, 79 %; P < 0·01) and was 22 % or 8·4 pmol/l lower after weight gain in cats fed the HCLP diet (95 % CI 2, 37 % lower; P = 0·03; significance of interaction P < 0·01). Peak insulin concentration was 48 % or 64·2 pmol/l higher after weight gain in cats fed the LCHP diet (95 % CI 24, 78 %; P < 0·01), but did not change significantly (mean peak was 0·6 pmol/l lower) after weight gain in cats fed the HCLP diet (estimated change 0 %; 95 % CI − 16, 18 %; P = 0·96; significance of interaction P < 0·01). Mean insulin concentration increased 46 % or 31·2 pmol/l after weight gain in cats fed the LCHP diet (95 % CI 25, 71 %; P < 0·01), but did not change significantly (mean concentration was 2·4 pmol/l lower) with weight gain in cats fed the HCLP diet (estimated change 2 %; 95 % CI − 17, 15 %; P = 0·77; significance of interaction P < 0·01).

Although mean insulin concentration increased 46 % with an average of 37 % weight gain in cats fed the LCHP diet, the HCLP diet in lean cats resulted in similar mean plasma insulin concentration compared with cats fed the LCHP diet after weight gain (Tables 4 and 6; Fig. 2(a) and (b)). Estimated percentage difference in lean cats fed the HCLP diet relative to cats after 37 % mean weigh gain fed the LCHP diet was 5 % lower (95 % CI − 29, 26 %; P = 0·70).

Effects of diet on insulin sensitivity and glucose effectiveness

Insulin sensitivity did not differ significantly between the diets either when cats were lean (P = 0·39) or after weight gain (P = 0·84; Tables 4 and 6). Insulin sensitivity did not change significantly with weight gain (P = 0·90), and there was no significant interaction between phase and diet (P = 0·23).

There was no significant difference in glucose effectiveness between the diets when cats were lean (P = 0·85); however, glucose effectiveness was significantly higher after weight gain in cats fed the HCLP diet compared with cats fed the LCHP diet (P = 0·04; Tables 4 and 6). Glucose effectiveness increased significantly with weight gain (P = 0·03). There was no significant interaction between phase and diet (P = 0·77).

Energetic efficiency of weight gain

The amount of energy required to maintain the body weight within 95–105 % of initial weight during the stable-weight phase was significantly less for cats fed the LCHP diet compared with cats fed the HCLP diet. Cats fed the LCHP diet ate on average 2·24 g less of food/kg body weight per d than cats fed the HCLP diet (95 % CI 0·39, 4·09; P = 0·02), equivalent to 41·8 kJ/kg body weight per d less energy (95 % CI 16·0, 67·6; P < 0·01). Energy intake averaged 178·1 kJ/kg body weight per d for the LCHP diet and 220·2 kJ/kg body weight per d for the HCLP diet.

In the weight-gain phase of the study, over 8 weeks of ad libitum feeding, the average food and energy intakes were similar in both groups. Food and energy intakes were 24 g/kg per d and 318 kJ/kg per d in the LCHP group, and 25 g/kg per d and 346 kJ/kg per d in the HCLP group of cats. Cats fed the LCHP diet ate on average 0·73 g of food less/kg body weight per d than cats fed the HCLP diet, a difference which was not significant (95 % CI − 3·39, 4·86; P = 0·71). Similarly, cats fed the LCHP diet consumed on average 31·8 kJ/kg body weight per d less than cats fed the HCLP diet (95 % CI − 26·30, 89·84; P = 0·26).

The LCHP diet resulted in greater energetic efficiency for body-weight gain: mean values were 52 845 kJ/kg weight gain v. 100 377 kJ/kg weight gain for the LCHP and HCLP diets, respectively. Cats fed the LCHP diet required on average 34 696 kJ less to gain 1 kg in body weight than cats fed the HCLP diet (95 % CI 19 663, 49 728; P < 0·01).

During the weight-gain phase, when food intake increased by 57 %, thirteen out of the sixteen cats (81 %) fed the HCLP diet developed diarrhoea. Faecal tests of some cats for parasites and potentially pathogenic bacteria were negative, and the diarrhoea did not resolve despite feeding a new batch of food and changing the source of protein from poultry to beef. Of these cats with diarrhoea, two cats that had constant watery diarrhoea were removed from the study. In all cats with diarrhoea, including the cats that were removed from the study, the diarrhoea resolved within 24 h after commencement of feeding the LCHP diet ad libitum.

Discussion

Based on the present results, there were a number of noteworthy findings. First, when fed ad libitum, a LCHP diet resulted in greater weight gain than a HCLP diet. This is in agreement with a previous study that evaluated the effect on weight gain in gonadectomised cats of low- and high-carbohydrate diets with similar amounts of protein and varying in fat content. In that study, weight gain after 17 weeks of ad libitum feeding was significantly higher in cats fed diets lower in carbohydrate (3 and 22 % ME) and higher in fat (64 and 44 % ME, respectively) compared with cats fed diets with high (57 % ME) and moderate (41 % ME) carbohydrate content and lower in fat (9 and 25 % ME, respectively)(Reference Backus, Cave and Keisler14). In fact, weight gain increased linearly with dietary fat content (% ME)(Reference Backus, Cave and Keisler14). However, the lowest carbohydrate diet had 90 % greater energy density than the highest, confounding the findings. The energy densities of the diets used in the present study were similar. Therefore, the present results increase confidence that when fed ad libitum, LCHP diets result in greater weight gain compared with HCLP diets, even when diets are of comparable energy density.

We hypothesise that the lower weight gain associated with the HCLP diet might result from several factors. First, although the energy densities were similar, the proportion of energy from fat was slightly lower in the HCLP diet (28 v. 30 % ME). Second, cats are reported to limit their carbohydrate intake, and this ‘ceiling’ effect on carbohydrate intake might have limited body-weight gain in our high-carbohydrate-fed cats(Reference Hewson-Hughes, Hewson-Hughes and Miller26). However, in the ad libitum phase, the cats in the present study consumed amounts of carbohydrate twice that reported for the carbohydrate ceiling in cats (mean 624 v. 300 kJ/d). It is possible that this higher carbohydrate intake in our cats reflects a longer adaptation period (12 weeks in the present study v. 1 week in the reported study) and/or the need to meet minimum protein requirements. A third hypothesis for the lower weight gain is that the energy bioavailability of the HCLP diet was substantially less than that of the LCHP diet. Loose stools were observed in the majority of cats given the HCLP diet during the weight-gain phase, and this might indicate there was fermentation of substrate that otherwise should have been available for absorption and utilisation of energy.

An important finding from the study was that the greater weight gain occurred because of greater energy efficiency associated with the LCHP diet. Cats eating the LCHP diet required significantly less energy (kJ/kg) to maintain their body weight when fed at maintenance energy requirements, and their energetic efficiency for body-weight gain was higher. The finding that when fed ad libitum, cats in the LCHP group consumed a similar amount of energy/kg body weight per d to cats eating the HCLP diet, but gained more weight, is in contrast to findings in human subjects where LCHP diets (Atkins diets) are associated with reduced energy intake and subsequently greater weight loss than high-carbohydrate diets(Reference Wylie-Rosett and Davis27). The findings in the present study are unlikely to be the result of marginal protein content in the HCLP diet because lean mass as measured by dual-energy X-ray absorptiometry did not change significantly from baseline at any time point over the 3 months (mean total lean mass was 2·4 kg before and after consuming the HCLP diet for 12 weeks).

Notably in the present study, 81 % of cats fed the HCLP diet ad libitum developed diarrhoea, suggesting that feeding excessive quantities of starch is not well tolerated in cats. Dietary carbohydrate has been reported to cause gastrointestinal disturbances in cats due to its osmotic effect if the amount eaten exceeds the digestive capacity of the small intestine(Reference Kienzle3, Reference Kienzle28), which has been reported to occur when carbohydrate content exceeds 40 % on a DM basis(Reference Meyer and Kienzle29). The National Research Council (USA) considers the adverse effects of carbohydrate in cats to include loose stools, elevated faecal water content and frequent defaecation(30). The findings in the present study are consistent with faecal quality data provided by the manufacturer from a digestibility trial following the Association of American Feed Control Officials' guidelines using the same high-carbohydrate diet used in the present study. At maintenance energy requirements, six adult cats (aged 1–8 years) were fed the HCLP diet and consumed 97 % of the amount offered. Faecal quality was poor based on 37·5 % unacceptable faeces, consisting of loose stools and diarrhoea with only 2·8 % ideal faeces. The carbohydrate source of the HCLP diet used in the present study was mainly wheat starch. However, it is unlikely that the wheat contributed to diarrhoea, because faecal quality data provided by the manufacturer for the same diet as the baseline diet (carbohydrate 37 % ME), but with wheat as the carbohydrate source, were associated with 0 % of unacceptable faeces. As both diets in the present study had very similar apparent digestibility scores, poor total digestibility of the HCLP diet does not explain the diarrhoea. However, it should be noted that apparent digestibility measures total intestinal tract digestibility and represents the combination of starch digested by mammalian enzymes and digestion of undigested starch in the colon by bacteria.

Previous studies have shown that cats are not adapted to use carbohydrate efficiently as a source of energy(Reference Kienzle28). Cats lack salivary amylase(Reference Herdt and Cunningham31) and have low activity of intestinal enzymes that break down carbohydrates, such as intestinal amylase, and disaccharidases(Reference Kienzle2, Reference Kienzle4, Reference Case, Carey and Hirakawa32). When fed at maintenance energy requirements, the HCLP diet did not cause diarrhoea; intolerance was only clinically evident during ad libitum feeding when the amount of carbohydrate eaten daily increased by 57 %. The resultant diarrhoea has been reported to be generally associated with the low activity of primary or secondary disaccharidases in cats(Reference Meyer and Kienzle29). Clinically, this may only be seen in cats being fed a high-carbohydrate diet and eating to excess during a rapid weight-gain phase, for example after neutering or in a newly adopted underweight cat, and would be expected to resolve over time as food intake stabilises towards maintenance levels.

A second finding is that most of the additional energy consumed by cats in both dietary groups during the ad libitum feeding resulted in increased fat deposition, which was predominantly external to the abdomen and presumably subcutaneous fat. This is in agreement with a previous study that evaluated the effect of diets of different composition on fat mass in gonadectomised cats(Reference Nguyen, Dumon and Siliart33). In the present study, total lean mass also increased with weight gain in the LCHP group. The increase in lean mass occurred in smaller proportion relative to the proportional increase in fat mass, which is in agreement with previous findings in human subjects that fat mass and lean mass change in the same direction as weight changes, with fat mass being more responsive to weight change than lean mass(Reference Forbes34, Reference Newman, Lee and Visser35)

Third, in contrast to the adverse effects on body weight of feeding a LCHP diet ad libitum, if fed at maintenance energy requirements, a LCHP diet might be beneficial for cats with a combination of risk factors for diabetes such as aged, obese, male cats, because of the smaller increase in plasma glucose and insulin concentrations after a meal compared with cats fed a HCLP diet. The present results demonstrated that in lean cats, the LCHP diet results in lower mean and peak glucose and insulin concentrations for at least 18 h after eating compared with the HCLP diet. This is in agreement with results from a recent study in cats fed a diet with 41 g/100 g carbohydrate compared with diets with lower amounts of carbohydrate (31 and 21 g/100 g)(Reference Hewson-Hughes, Gilham and Upton7). Nevertheless, in the present study, to maintain the energy content of the diets when the carbohydrate content of the diet was changed, a compensatory change in protein was made. The observed effects on postprandial plasma glucose and insulin concentrations could be due to changes in protein content, because amino acids stimulate insulin secretion and are a substrate for gluconeogenesis(Reference Floyd, Fajans and Conn36, Reference Daniel, Pratt and Spargo37). However, results from studies in human subjects, cats and dogs indicate that carbohydrates are the principal nutrients involved in the postprandial changes in plasma glucose and insulin(Reference Hewson-Hughes, Gilham and Upton7, Reference Nguyen, Dumon and Buttin38, Reference Wolever and Bolognesi39).

Carbohydrate source might have had some influence on postprandial glucose and insulin concentrations in the present study. The difference between rice and maize/sorghum as carbohydrate sources has been previously shown to have only minor effects on postprandial blood glucose concentration, compared with the marked effect resulting from differences in the total amount of carbohydrate (Farrow HA, Rand JS and Sunvold GD (2002), unpublished results)(Reference Hewson-Hughes, Gilham and Upton7, Reference Appleton, Rand and Priest40). However, a recent study of novel carbohydrate sources such as lentil and cassava flour demonstrated that the glucose and insulin increase after eating is minimum compared with corn(Reference de-Oliveira, Carciofi and Oliveira41), which was the carbohydrate source used in the LCHP diet in the present study. The HCLP diet used in the present study had wheat as the carbohydrate source, and there are no data in cats demonstrating the glycaemic response to wheat. It is possible that wheat results in a higher postprandial glycaemic response than maize and that might also have contributed to the magnitude of increase in glucose and insulin in the HCLP diet.

A fourth finding was that after an average weight gain of 37 %, cats eating the LCHP diet had a similar mean glucose concentration over 24 h as lean cats eating the HCLP diet. This suggests that a HCLP diet produces similar adverse effects on mean postprandial glucose concentrations to the effects of a substantial short-term weight gain. Of more concern with respect to the potential to predispose to diabetes, the HCLP diet in lean cats resulted in similar mean plasma insulin concentration for at least 15 h after eating compared with the postprandial increase in insulin concentration associated with a mean 37 % weight gain in cats eating a LCHP diet. Chronic hyperglycaemia increases the demand on the β-cells to secrete insulin, and chronic hyperinsulinaemia is associated with eventual β-cell failure and type 2 diabetes(Reference Porte15) The International Diabetes Federation defines postprandial hyperglycaemia in humans as a plasma glucose concentration of greater than 7·8 mmol/l(Reference Ceriello and Colagiuri42), and individual cats in the present study fed the HCLP diet had mean glucose concentrations above this level. This suggests that if fed long-term, high-carbohydrate diets could potentially predispose to type 2 diabetes in susceptible cats, that is, cats with underlying low insulin sensitivity, for example aged, obese or Burmese cats, or those with underlying loss of β-cells from islet amyloid deposition.

In a study of feline patients in the UK, consumption of wet diets (lower in carbohydrate) and dry diets (higher in carbohydrate) were both associated with greater risk for diabetes compared with a mixed diet containing both wet and dry foods(Reference McCann, Simpson and Shaw43). Cats fed wet diets were three times more likely to develop diabetes than cats fed mixed diets; cats fed dry diets had two times the risk. This is consistent with the findings from the present study, because both weight gain and consumption of a HCLP diet were associated with higher mean glucose and insulin concentrations over 24 h compared with glucose and insulin concentrations in lean cats fed the LCHP diet. Based on the results of the UK study, it has been suggested that the adverse effects of obesity resulting from ad libitum feeding of low-carbohydrate diets (higher in fat) and the adverse effects of chronically higher demand for insulin secretion resulting from feeding high-carbohydrate diets both predispose to diabetes, with the obesity-potentiating effect posing greater risk. To further investigate the role of diet in predisposing to feline diabetes, additional well-designed dietary studies are required in which the confounding effects of ad libitum feeding and obesity have been controlled for, and sufficient numbers of cats are enrolled to have the statistical power to detect differences if they were present.

Insulin sensitivity was not different between diets or between lean and overweight cats. Insulin sensitivity is measured in the fasted state, which might minimise a dietary effect if present. Currently, there are no methods available to measure insulin sensitivity in the postprandial state. It is possible that moderate (26 and 31 % total body fat), short-term weight gain (8 weeks in the present study) may have different effects on insulin sensitivity to more pronounced weight gain over a longer period. In contrast to the present study where none of the cats were classed as obese, insulin sensitivity was halved when cats became obese over 10 months(Reference Appleton, Rand and Sunvold13). It is also possible that because most of the fat gained was outside the abdomen, it might have diminished the effect on insulin sensitivity(Reference Lindmark, Lönn and Wiklund44, Reference Pietiläinen, Rissanen and Kaprio45).

Glucose effectiveness measures the ability of glucose per se, under basal insulin conditions, to promote its own disposal through mass action into tissues and suppress endogenous glucose production(Reference Finegood, Hramiak and Dupre46, Reference Best, Kahn and Ader47). In healthy human subjects, 50 % of the glucose disposal during a glucose tolerance test is due to glucose effectiveness(Reference Best, Kahn and Ader47). Glucose effectiveness is enhanced with increased plasma insulin or glucose concentrations, and a 4-fold increase in insulin or a doubling of glucose concentrations result in a similar enhancing effect(Reference Best, Kahn and Ader47, Reference Roden, Perseghin and Petersen48). Although glucose effectiveness was not significantly different between the diets during the stable-weight phase, it increased with weight gain, and was significantly higher in cats fed the HCLP diet. Because insulin concentrations were not different between the diets after weight gain, but peak glucose concentration was significantly higher in cats fed the HCLP diet, it suggests that the higher glucose effectiveness with weight gain reflected the higher glucose concentration (mean peak 7·2 v. 9·2 mmol/l). The lower fasting glucose concentration in the HCLP group after weight gain might reflect increased glucose effectiveness.

Limitations of the study were that the diets were commercially available diets which had other micronutrient differences between them, and it is possible that other unknown effects could have accounted for some of the differences observed. The aim of the present study was to document the consequences of choosing a commercially available, HCLP diet over a LCHP diet. Although premium feline dry diets contain lower amounts of carbohydrate, the HCLP diet used in the present study is typical of the low-priced dry cat foods available in supermarkets in Australia. The LCHP diet is lower in carbohydrate than typical premium maintenance feline diets, but is at the high end of prescription LCHP diets recommended for diabetic cats. To further compare low- and high-carbohydrate diets, studies of diets identical except for macronutrient amount should be compared. In addition, diets with lesser amounts of carbohydrate (e.g. 40 % ME) need to be investigated to determine whether differences in energetic efficiency are also evident when more moderate levels of carbohydrate are fed ad libitum to promote weight gain. Although ad libitum feeding is the most common feeding method employed by owners of cats, it clearly promotes weight gain, which is a risk factor for a number of feline diseases including diabetes mellitus and reduces life span, and therefore is not recommended(Reference Scarlett and Donoghue12, Reference Lund, Armstrong and Kirk49).

Conclusions

In cats fed to maintain ideal body weight, HCLP diets result in higher postprandial glucose and insulin concentrations compared with LCHP diets. The effects on postprandial plasma glucose and insulin concentrations in lean cats fed the HCLP diet are similar to the effects on glucose and insulin concentrations associated with the levels of weight gain observed in the present study. In cats fed ad libitum, the LCHP diet promotes greater weight gain than the HCLP diet, but when fed at maintenance energy requirements, this diet may reduce the demand on β-cells to secrete insulin. When consumed ad libitum at amounts that result in weight gain, the HCLP diet results in diarrhoea in a majority of cats, and is associated with reduced energetic efficiency for weight gain.

Acknowledgements

The authors would like to thank the WALTHAM Centre for Pet Nutrition for the financial support, and David Alexander, Lyn Knott, Maree Maher, Philippa Williams, Helen Kwan, Rebekah Scotney, Melita Watkins and Karen Tuck for their valuable assistance. This study was supported by an Australian Research Council Linkage Grant and the WALTHAM Centre for Pet Nutrition (Masterfoods Australia and New Zealand). M. C. conducted the study as part of her PhD thesis, being involved in the design of the study, data collection, analyses of the results, interpretation of the data and writing of the manuscript; J. S. R. was involved in the study design, analyses of the results, interpretation of the data and writing of the manuscript; J. M. M. was involved in the statistical analyses of the results, interpretation of the data and writing of the manuscript; J. M. R. from the Waltham Centre for Pet Nutrition was involved in assisting with the study design, interpretation of the data, writing of the manuscript, and the decision to submit it for publication. M. C., J. S. R. and J. M. M. report no real or perceived vested interests that relate to this manuscript (including relationships with the granting body or other entities whose products or services are related to topics covered in this manuscript) that could be construed as a conflict of interest. J. M. R. declares that, as an employee of Mars Incorporated, he has potential conflict of interest, since all diets used in the study were Mars products.

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Figure 0

Table 1 Diet analyses, main ingredients, digestibility and energetic density of each diet

Figure 1

Table 2 Timeline of feeding and test weeks

Figure 2

Table 3 Body weight, total and abdominal fat and lean masses measured at the beginning and at the end of the stable-weight phase, and at the end of the weight-gain phase, after 8 weeks of ad libitum feeding(Mean values, percentages, standard deviations and 95 % confidence intervals)

Figure 3

Table 4 Fasting, peak and mean concentrations of plasma glucose and insulin during a 24 h meal-feeding test, insulin sensitivity and glucose effectiveness based on the minimal model analysis of the insulin-modified intravenous glucose tolerance test at the end of the stable-weight phase, after lean cats had been fed a low carbohydrate, high protein or high carbohydrate, low protein diet maintaining their body weight for 3 weeks(Mean values, standard deviations, ranges and 95 % confidence intervals)

Figure 4

Fig. 1 Comparison of the changes in plasma glucose concentration in the low carbohydrate, high protein (●) and high carbohydrate, low protein (○) dietary groups before and after weight gain. (a) End of stable-weight phase and (b) end of weight-gain phase. Values are means, with standard errors of the mean represented by vertical bars.

Figure 5

Table 5 Times (h) to exceed fasting concentration, times to peak and times to return to fasting concentration for plasma glucose and insulin during the 24 h meal-feeding test at the end of the stable-weight phase, after lean cats had been fed either the low carbohydrate, high protein or the high carbohydrate, low protein diet maintaining their body weight for 3 weeks(25th percentiles, median values, 75th percentiles)

Figure 6

Table 6 Fasting, peak and mean concentrations of plasma glucose and insulin during a 24 h meal-feeding test, insulin sensitivity and glucose effectiveness based on the minimal model analysis of the insulin-modified intravenous glucose tolerance test at the end of the weight-gain phase, after cats had been fed a low carbohydrate, high protein or high carbohydrate, low protein diet ad libitum for 8 weeks(Mean values, standard deviations, ranges and 95 % confidence intervals)

Figure 7

Table 7 Times to exceed fasting concentration, times to peak and times to return to fasting concentration for plasma glucose and insulin during the 24 h meal-feeding test at the end of the weight-gain phase, after cats had been fed the low carbohydrate, high protein or the high carbohydrate, low protein diet ad libitum for 8 weeks(25th percentiles, median values, 75th percentiles)

Figure 8

Fig. 2 Comparison of the changes in plasma insulin concentration in the low carbohydrate, high protein (●) and high carbohydrate, low protein (○) dietary groups before and after weight gain. (a) End of stable-weight phase and (b) end of weight-gain phase. Values are means, with standard errors of the mean represented by vertical bars.