Animals and diets

The animal experiments used 150 male Sprague–Dawley rats that were approximately 240 g in weight and were purchased from the Beijing Vital River Laboratory Animal Center. Rats were caged individually and were maintained under controlled temperature (22±2°C), humidity and airflow condition, with a 12-h on–off light cycle as described by Rutherfurd et al. ⁽ Reference Rutherfurd, Fanning and Miller ^{3 )}. Adequate measures were taken to minimise the pain or discomfort of the rats, and we used the smallest possible number of animals. The study was reviewed and approved by the Institutional Animal Ethics Committee at Jiangnan University (JN. No. 20170930k1201105 [36]). All animals were maintained according to local regulations and guidelines.

A total of eleven semisynthetic wheat starch-based diets (Table 1) were formulated to contain 100 g/kg CP, which was the sole protein source. To meet the requirements for growing rats, we added vitamins and minerals. A total of 3 g/kg of titanium dioxide was included in each diet as an indigestible marker. Purified sucrose, soyabean oil and cellulose were mixed in a ratio of 10:5:3 (180 g/kg DM). To maintain a dietary CP concentration of 100 g/kg for low-protein foods with CP concentration of <150 g/kg DM, the test ingredient was diluted with cellulose and soyabean oil (1:0·6); for foods with CP concentration of <100 g/kg DM, the test diet consists of the test ingredient, vitamin/mineral mixture and titanium dioxide^{( 20 )}. The ingredient compositions of the basal and test diets are shown in Table 1. A protein-free-based diet was prepared for rats to determine the amount of endogenous loss of AA in the ileal content⁽ Reference Moughan and Rutherfurd ^{21 )}. A basal diet containing 100 g/kg protein was also formulated using casein as the sole source of protein⁽ Reference Rutherfurd and Moughan ^{22 )}.

Table 1 Ingredient composition of the experimental diet (g/kg DM)

* The vitamins and trace elements are as follows: 250 mg retinol; 1·8 mg cholecalciferol; 1185 mg α-tocopherol; 1808 mg thiamine; 312 mg riboflavin; 2338 mg niacin; 2058 mg pantothenic acid; 312 mg pyridoxine; 1·8 mg cyanocobalamin; 125 mg phylloquinone; 93·9 mg folic acid; 4·56 g Mn; 10·29 g Fe; 904 mg Cu; 3273 mg Zn; 41 mg iodine; 7·5 mg Se; 39 mg Co.

† The mineral mix of the diet includes 25 g CaPO₄, 5·3 g CaCO₃, 3·6 g NaCl, 12·5 g KCl and 3·6 g MgSO₄.

Experimental design

The rats (n 150) were randomly divided into 10 groups (n 15/group) as follows: brown rice group, polished rice group, buckwheat group, oats group, proso millet group, foxtail millet group, tartary buckwheat group, adlay group, whole wheat group and protein-free-based diet group. All rats were initially fed a standard basal diet for 7 d. After 1 week of acclimatisation period, the experimental groups received each diet in Table 1 for 7 d. Each rat received its respective diet in nine hourly meals (08.30–16.30 hours) daily. The diet was freely available for 10 min at each meal time. Water was also freely available. On the 14th day of the study, each rat was killed 5 h after the first meal through asphyxiation with CO₂ gas⁽ Reference Rutherfurd, Fanning and Miller ^{3 ,} Reference Rutherfurd and Moughan ^{23 )}. Ileal contents were immediately collected from the terminal 20 cm of ileum. Given that the ileal content of each rat is insufficient for the AA detection through HPLC⁽ Reference Rutherfurd and Moughan ^{22 )}, three ileum contents were mixed into one sample in each group (n 5). All ileal content samples were freeze-dried and frozen (–20°C) while awaiting chemical analysis.

Chemical analysis

CP content was determined by rapid N cube (NY/T 2007–2011) using a N-to-protein conversion factor of 6·25. The AA contents were determined in triplicate 5-mg samples following hydrolysis in 500 µl of constant-boiling HCl (6 mol/l) for 24 h at 110±1°C in a hydrolysis tube⁽ Reference Rutherfurd and Gilani ^{24 )}. The liberated AA were derived with 6-aminoquinolyl-N-hydroxysuccinimidyl carbamate, and α-aminobutyric acid was used as the internal standard. The derivatives were separated on a Waters E2695 HPLC system equipped with a C18 column (150 mm×4·6 mm, 5·0 µm; Agilent) and quantified using Waters 2475 fluorescence detector at 395 nm emission and 250 nm excitation. To determine cysteine and methionine, we used performic acid oxidation at 0°C for 16 h, followed by neutralisation with HBr; then, we applied hydrolysis as described above. The concentration of titanium in the diets and ileal samples was determined through the method described by Short et al. ⁽ Reference Short, Gorton and Wiseman ^{25 )}. The samples were ashed, then digested in 60 % (v/v) sulfuric acid and finally added to 30 % hydrogen peroxide. Absorbance at 410 nm was measured. Tryptophan (Trp) was determined using the method described by Rutherfurd & Gilani⁽ Reference Rutherfurd and Gilani ^{24 )}. Free AA molecular weights were used for the calculation of the weight of each AA.

Data analysis

AA and CP contents in the terminal ileal digesta and the TID of AA were calculated by using the equation given by Rutherfurd et al. ⁽ Reference Rutherfurd, Bains and Moughan ^{26 )}. In addition, the endogenous ileal AA flows were determined for rats fed the protein-free diet⁽ Reference Rutherfurd, Cui and Goroncy ^{27 )}.

Apparent and true ileal AA digestibility was calculated using the following equations (units are g/kg DM intake)⁽ Reference Stein, Seve and Fuller ^{6 ,} Reference Cervantes-Pahm, Liu and Stein ^{28 )}:

$${\rm AID}_{{{\rm AA}}} {\equals}1\!-\!\left( {\left( {{\rm AA}_{{{\rm digesta}}} /{\rm AA}_{{{\rm diet}}} } \right){\times}\left( {{\rm Ti}_{{{\rm diet}}} /{\rm Ti}_{{{\rm digesta}}} } \right)} \right){\times}100,$$

where AID_AA is the AID of AA (%), AA_digesta is the concentration of AA in the ileal digesta DM, AA_diet is the concentration of AA in the diet DM, Ti_diet is the concentration of Ti in the diet DM and Ti_digesta is the concentration of Ti in the ileal digesta DM.

$${\rm TID}_{{{\rm AA}}} {\equals}{\rm AID}{\plus}\left( {\left( {{\rm IAA}_{{{\rm end}}} /{\rm AA}_{{{\rm diet}}} } \right){\times}100} \right),$$

where IAA_end is the ileal endogenous AA losses.

$${\rm DIAA}\;{\rm reference}\;{\rm ratio}{\equals}{{{\rm mg}\;{\rm of}\;{\rm the}\;{\rm digestible}\;{\rm dietary}\;{\rm indispensable}\;{\rm AA}\;{\rm in}\;{\rm 1}\;{\rm g}\;{\rm of}\;{\rm the}\;{\rm test}\;{\rm protein}} \over {{\rm mg}\;{\rm of}\;{\rm the}\;{\rm dietary}\;{\rm indispensable}\;{\rm AA}\;{\rm in}\;{\rm 1}\;{\rm g}\;{\rm of}\;{\rm the}\;{\rm reference}\;{\rm protein}}}$$

where the reference protein indispensable AA profile was the AA requirement pattern for the 0·5–3 years old child^{( 15 )}.

DIAAS was calculated using the following equation^{( 15 , 20 )}:

$$\eqalign{ {\rm DIAAS }\left( {\rm \,\&#x0025;\,} \right) &#x0026; {\rm {\equals} 100{\times}lowest}\,\,{\rm value}\,\,{\rm of}\,\,{\rm the}\,\,{\rm digestible} \ {\rm indispensable} \cr &#x0026; \quad{\rm AA}\,\,{\rm reference}\,\,{\rm ratio}{\rm .}$$

Statistical analysis

Calculation of sample size was performed using the ‘resource equation’ method, as described by Charan & Kantharia⁽ Reference Charan and Kantharia ^{29 )}, with a power of 80 % and significance of 5 %. Results were expressed as mean values with their standard errors. The Shapiro–Wilk comparison normality test was used to assess the distribution of all variables. Comparisons for normally distributed data between the two groups were conducted using two-tailed t test and one-way ANOVA followed by Tukey’s significance test for multiple comparisons. Mann–Whitney U and Kruskal–Wallis tests were used for non-parametric analysis when data were non-normally distributed. A P value of <0·05 was considered significant. All statistical calculations were performed on SPSS 21.0 data processing software (SPSS Inc.).