Experimental methods

A panel of seven healthy adult neutered dogs of various breeds was studied. Within the panel were three males and four females, ranging in age from 1 year and 6 months to 4 years and 3 months, body weights ranging from 9·1 to 30·7 kg (mean 18·9 kg). The study took place at the Verden Pet Centre (Mars Petcare) and all methods were conducted in accordance with paragraph 11 of the Animal Protection Law as approved by the Veterinary Inspection Office, Germany. Dogs were housed in pairs throughout the study in kennels equipped with indoor and outdoor runs. Each dog received a daily socialisation period of 40 min and had ad libitum access to water throughout the 11 d main study.

To investigate the energy density of the dog chew (PEDIGREE^® Dentastix™; Mars Petcare), the product was rendered nutritionally adequate for solus feeding (i.e. the test product represented the only nutrient source) by the addition of vitamins and minerals. The tartar sequestrant sodium tripolyphosphate (STPP) was removed from the product to ensure appropriate P levels. A single batch of this adapted product (‘test product’) was manufactured using a twin-screw extruder and cut into kibbles.

A preliminary study was conducted to assess faeces quality and general health of the dogs in association with solus feeding of the test product. The study consisted of a 2 d pre-feed of standard diet (PEDIGREE^® Adult chunk in loaf) followed by a 3 d period of feeding the test product solus. Faeces were scored throughout the 5 d study until 12.00 hours on day 6, using a grading system of 1 to 5 according to the method of Moxham⁽ Reference Moxham ^{3 )}.

The main study comprised a 3 d pre-feed phase where dogs received standard diet as described previously, followed by an 8 d phase of feeding the test product solus. Dogs received the test product as two meals per d, to provide their individual daily energy requirement according to the following equation: 95 kcal/kg body weight^0·75 per d (397 kJ/kg body weight^0·75 per d). During the adaptation phase (4–6 d), no samples of faeces or diet were collected to allow for complete transition of test product through the digestive tract. During the collection phase (7–11 d), faeces were collected daily, pooled for each dog and stored at −20°C prior to analysis. Food intakes and refusals were recorded daily.

Faeces and test diet samples were analysed by a commercial laboratory (Eurofins Institute Dr Appelt Southwest GmbH) for proximate nutrient content (moisture, protein, fat, fibre and inorganic matter). Prior to analysis, diet and faeces were ground through a 1 mm screen and homogenised. Protein was analysed according to the Kjeldahl method. Fat and fibre contents were determined according to § 64 LFGB-Methode F 0003. (This reference corresponds to EG 152/2009 and VDLUFA Bd. III 4.1.1.) Ash content was determined via treatment in a muffle furnace at 550°C for 5 h. N-free extract (NFE) was calculated as 100 minus the sum of percentages of moisture, protein, fat, ash and fibre. Bomb calorimetry was used to determine gross energy (GE).

Calculations and statistical analysis

PME was calculated using proximate analysis in combination with modified Atwater factors, using the following equations:

$$\eqalign{& {\rm GE}\;{\rm (kJ/g) = }\,({\rm 23}{\rm \cdot 85}\times {\rm g}\;{\rm protein})+\left( {{\rm 39}{\rm \cdot 33} \times {\rm g}\;{\rm fat}} \right)\, \cr & \quad+\,{\rm 17}{\rm \cdot 15} \times {\rm g \;(NFE + crude}\,\,{\rm fibre)} \cr & {\rm \% }\;{\rm Energy}\;{\rm digestibility}\,{\rm = }\,{\rm 91}{\rm \cdot 2}{\rm - (}{\rm 1}{\rm \cdot 43} \times {\rm \% }\;{\rm crude}\;{\rm fibre}\;{\rm in}\;{\rm DM}{\rm )} \cr & {\rm DE\;(kJ/g)}\,{\rm = }\,{\rm GE} \times {\rm \% }\;{\rm energy}\;{\rm digestibility/100} \cr & {\rm PME\;(kJ/g)}\,{\rm = }\,{\rm DE}{\rm - (}{\rm 4}{\rm \cdot 35} \times {\rm g}\;{\rm protein}{\rm )}} $$

Digestibility coefficients for DM, energy, protein, fat, ash, organic matter and NFE were determined for each dog as apparent digestibility ((consumed − faecal)/consumed). From these, means and standard deviations were calculated using Microsoft^® Excel^® 2013 (version 15.0.4911.1000). ME was calculated by applying a correction factor of 1·25 kcal/g (5·23 kJ/g) digestible crude protein to the calculated digestible energy (DE) to account for energy lost in urine^{( 4 )}. Energy release from hindgut fermentation was not taken into account as this is considered to be negligible in dogs⁽ Reference McKay and Eastwood ^{5 )}.