Sample collection and experimental design

Approximately 0.5 kg of fresh leaves of KL without stem were harvested for the sample collection. Samples of KL with old maturity were collected from 80–90 cm herbaceous-shrub plant in Bandung, Indonesia. In Bandung, annual precipitation ranges from 2500 to 3000 mm and temperature ranges from 24 to 28 °C (BMKG, 2013).

After collection, KL samples were stored at 4 °C overnight, oven dried at 60 °C for 24 h (F115, Binder GmbH, Tuttlingen, Germany), and ground to pass a 1 mm sieve using a laboratory mill (model SM100, Retsch GmbH, Haan, Germany). As a substrate for KL to be added to, three grass hays from temperate regions (grown in Germany and Switzerland) were selected based on their CP concentration to represent a wide range of qualities: hay with low quality (LQH), hay with medium quality (MQH) and hay with high quality (HQH). Hays were ground to pass a 1 mm sieve using the same mill as for KL. Samples of KL and each grass hay were incubated alone or in KL + grass hay combinations with four different inclusion levels of KL (i.e. 0, 50, 100 and 200 g/kg dry matter (DM)). The cows used as donor animals were housed in accordance with the German Animal Welfare legislation. All procedures for animal handling within the present study were performed according to the National Committee for the Protection of Animals Used for Scientific Purposes for the Federal Republic of Germany. The experimental diets were arranged in a completely randomized design in six replicates. The feedstuff combinations, i.e. diets, are presented in Table 1.

Table 1. Ingredient composition and calculated chemical composition (n = 2) of the experimental diets

ADFom, acid detergent fibre expressed exclusive of residual ash; aNDFom, neutral detergent fibre assayed with a heat-stable amylase and expressed exclusive of residual ash; DM, dry matter; FM, fresh matter; Lignin (sa), lignin determined by solubilization of cellulose with sulphuric acid; NFC, non-fibrous carbohydrate.

^a Cellulose = ADFom – Lignin (sa); hemicellulose = aNDFom – ADFom; NFC = 1000 – (aNDFom + crude protein + ether extract + ash).

Chemical analyses

Chemical composition of the individual sample was determined according to the Association of German Agricultural Analytic and Research Institutes (Verband Deutscher Landwirtschaftlicher Untersuchungs- und Forschungsanstalten, 2007). The DM concentration was determined by oven-drying at 105 °C for 24 h (method 3.1) and ash concentration was determined by incinerating samples at 550  °C for 5 h (method 8.1). The N concentration was determined by Kjeldahl procedure (method 4.1.2) and CP was calculated as N×6.25. Ether extract (EE) concentration was analysed using method 5.1.1. Neutral detergent fibre, assayed with a heat-stable amylase and expressed exclusive of residual ash (aNDFom), acid detergent fibre, expressed exclusive of residual ash (ADFom) and lignin determined by solubilization of cellulose with sulphuric acid (Lignin (sa)) concentrations were measured using an ANKOM200 Fibre Analyzer (Ankom Technology Corp., Macedon, NY, USA) according to methods 6.5.1, 6.5.2 and 6.5.3, respectively. Sodium sulphite was used for the aNDFom analysis. Concentration of hemicelluloses was determined by subtracting ADFom concentration from aNDFom concentration and concentration of cellulose by subtracting Lignin (sa) concentration from ADFom concentration (Rinne et al., Reference Rinne, Jaakkola and Huhtanen1997). All samples were analysed in duplicate for each chemical constituent and analysis repeated, if the coefficient of variation exceeded 5%.

Non-fibre carbohydrates (NFC) were calculated according to National Research Council (2001), as:

(1)$${\rm NFC} = 1000-( {{\rm aNDFom} + {\rm CP} + {\rm EE} + {\rm ash}} ) $$

where all nutrient concentrations are in g/kg DM.

Tannin bioassay

To investigate whether the KL sample contained tannins or not, an indirect approach was selected. Katuk leaves were evaluated using polyethylene glycol (PEG) supplementation in an in vitro GP experiment as mentioned by Jayanegara et al. (Reference Jayanegara, Togtokhbayar, Makkar and Becker2009). The PEG has a high affinity for tannins and makes tannins inactive by binding to them. Hence, KL samples (220–250 mg) were incubated without and with 750 mg PEG supplementation with 10 ml of rumen fluid and 20 ml of buffer solution (Menke et al., Reference Menke, Raab, Salewski, Steingass, Fritz and Schneider1979) using Hohenheim gas test (HGT; Makkar et al., Reference Makkar, Blümmel and Becker1995).

The syringes were placed in a rotor inside the incubator (39 °C) with about one rotation per minute. The GP was recorded after 48 h of incubation (GP₄₈). Blanks were prepared by incubating syringes containing rumen fluid and buffer solution, but without any sample. Katuk leave samples were incubated in triplicate in two different in vitro incubation runs. The difference between the in vitro GP with and without PEG supplementation is an indicator of tannin effect. The increase in gas on addition of PEG is a measure of tannin activity, where the protocol used was similar to that described in Makkar et al. (Reference Makkar, Blümmel and Becker1995).

Fibre fractionation and in vitro fibre digestibility

The fibre fractionation and in vitro fibre digestibility experiment were evaluated using the modified Tilley and Terry technique (Tilley and Terry, Reference Tilley and Terry1963; Robertson and Van Soest, Reference Robertson, Van Soest, James and Theander1981). For this, rumen fluid was collected from two rumen-fistulated Jersey cows, fed on a total mixed ration containing grass silage (180 g/kg DM), corn silage (167 g/kg DM), grass hay (184 g/kg DM), barley straw (21 g/kg DM), and concentrate mixture (426 g/kg DM), urea (2 g/kg DM) and mineral mixture (20 g/kg DM). The total mixed ration had a forage to concentrate ratio of 55:45 (on DM basis) and contained 148 g CP/kg DM. Rumen fluid was collected immediately before morning feeding and strained through two layers of cheesecloth into pre-warmed and isolated bottle. All laboratory handling of rumen fluid was carried out under a continuous flow of CO₂. The rumen fluid of both cows was mixed, homogenized and filtered using a nylon net (pore size 100 μm).

The ground initial sample (500 mg) was weighed into a 250 ml flask (Goering and Van Soest, Reference Goering and Van Soest1970). The rumen fluid (10 ml) and the buffer solution (40 ml) were added to each flask. The flasks were then placed in a preheated (39 °C) water bath under CO₂ positive pressure to ensure anaerobiosis, and incubated for 240 h, which corresponds to the maximum extent of fibre digestion in an anaerobic environment in vitro (Fox et al., Reference Fox, Tedeschi, Tylutki, Russell, Van Amburgh, Chase, Pell and Overton2004; Raffrenato and Van Amburgh, Reference Raffrenato and Van Amburgh2010; Raffrenato et al., Reference Raffrenato, Ross and Van Amburgh2018). Re-inoculation of the flasks with 10 ml rumen fluid and 40 ml buffer solution was conducted after 120 h of incubation to preserve the microbial activity during the whole incubation process (Palmonari et al., Reference Palmonari, Fustini, Canestrari, Grilli and Formigoni2014). Blanks were prepared by incubating flasks containing buffer and rumen fluid but without any sample to correct for any feed particles introduced into the in vitro system with the rumen fluid (Raffrenato et al., Reference Raffrenato, Ross and Van Amburgh2018). Each sample was incubated in triplicate in two runs resulting in six observations per experimental diet.

At the end of the incubation, the whole content of each flask was moved to a 600 ml beaker that was covered by a round cold-water condenser to minimize evaporation (Mertens, Reference Mertens2002) and determine the aNDFom concentration of the residue (Goering and Van Soest, Reference Goering and Van Soest1970). About 0.5 g of sodium sulphite and 50 ml of neutral detergent solution were added to each refluxing beaker and refluxed for 60 min at boiling temperature to create vigorous particle movement. After refluxing, the content of each beaker was filtered through crucibles (40 μm porosity, Duran™ Borosilicate Glass Filter Crucibles number 2, DWK Life Sciences, Wertheim, Germany) and the water removed with a vacuum pump. Filtered residues were dried in a forced-air oven (105 °C) for 3 h, and the weights of the crucibles were recorded. Ash correction was done by incineration of the residue at 550 °C for 4 h.

The in vitro neutral detergent fibre digestibility (IVNDFD of the incubated samples after 240 h; IVNDFD₂₄₀) was calculated as

(2)$${\rm IVNDF}{\rm D}_{ 240} = \displaystyle{{{\rm aNDFo}{\rm m}_{\rm r}{\rm \ndash aNDFo}{\rm m}_{\rm b}} \over {{\rm aNDFo}{\rm m}_{\rm i}}}$$

where aNDFom_r is the residual aNDFom after 240 h in vitro fermentation (g/kg DM), aNDFom_b is the blank correction after 240 h in vitro fermentation (g/kg DM) and aNDFom_i represents the initial aNDFom concentration from samples (g/kg DM).

The uNDF concentration (g/kg DM) after 240 h in vitro fermentation (uNDF₂₄₀) was calculated as

(3)$${\rm uND}{\rm F}_{ 240} \,( {{\rm g/kg\;DM}} ) = \displaystyle{{( {{\rm 1000\ndash IVNDF}{\rm D}_{ 240}} ) {\rm \;x\;aNDFo}{\rm m}_{\rm I}{\rm \;}} \over { 1000}}$$

where aNDFom_i (g/kg DM) is the aNDFom concentration of the sample (g/kg DM) and IVNDFD₂₄₀ is in vitro fibre digestibility (IVNDFD) of the incubated samples after 240 h.

The pdNDF concentration (g/kg DM) was calculated as

(4)$${\rm pdNDF\;}( {{\rm g/kg\;DM}} ) {\rm} = {\rm aNDFo}{\rm m}_{\rm i}{\rm \ndash \;uND}{\rm F}_{ 240}{\rm \;}$$

where aNDFom_i (g/kg DM) is the aNDFom concentration of the sample (g/kg DM) and uNDF₂₄₀ is the uNDF in the residue after 240 h in vitro fermentation (g/kg DM).

In vitro gas production, metabolizable energy and net energy for lactation

The HGT was performed according to Menke and Steingass (Reference Menke and Steingass1988) but modified regarding the incubation duration. Rumen fluid was collected from two castrated male adult Blackface sheep, fed on a standard diet of grass hay, a commercial compound feed and barley (650, 200 and 150 g/kg DM, respectively) that covered maintenance energy requirements. The animals never received tanniferous and/or tropical feeds before. Rumen fluid was collected immediately before feeding and strained through two layers of cheesecloth into pre-warmed and isolated bottle. All laboratory handling of rumen fluid was carried out under a continuous flow of CO₂.

The ground samples (220–250 mg) of the air-dried feedstuffs and the respective mixtures were accurately weighed into 100 ml glass syringes and the syringe pistons were lubricated with Vaseline and inserted into the syringes. Triplicates of syringes without substrate (blanks) and of standard hay and concentrate were included as laboratory controls. According to Menke and Steingass (Reference Menke and Steingass1988), GP from the blank was subtracted from all samples incubated to obtain the net GP. Subsequently, GP from the hay standard was divided by the measured net value of the hay standard to provide the correction factor. Similarly, GP from the concentrate standard was divided by the measured net GP of the concentrate standard. The average value of correction factor and concentrate standard was used for the adjustment. Each sample was incubated in triplicate in two different in vitro incubation runs. Incubations were repeated when gas volumes of the standards deviated by more than 10% and when coefficient of variation between repetitions exceeded 5% from the reference values.

Syringes were filled with 30 ml of medium consisting of rumen fluid (10 ml) and 20 buffer solution (20 ml) as described by Menke and Steingass (Reference Menke and Steingass1988), except that the concentration of NaHCO₃ was reduced to 33 g/l and that of (NH₄)HCO₃ increased to 6 g/l to prevent a shortage in N during prolonged incubation times. The syringes were placed in a rotor inside the incubator (39 °C) with about one rotation per minute. The GP was recorded after 2, 4, 6, 8, 12, 16, 24, 36, 48, 60, 72 and 96 h of incubation. The ME and net energy for lactation (NEL) values were calculated according to Menke and Steingass (Reference Menke and Steingass1988) as:

(5)$${\rm ME} = 2 .20 + 0{\rm .1357\ GP} + 0{\rm .0057\ CP} + 0{\rm .0002859\ E}{\rm E}^ 2$$

(6)$${\rm NEL} = 0 .54 + 0{\rm .0959\ GP} + 0{\rm .0038\ CP} + 0{\rm .0001733\ E}{\rm E}^ 2$$

where GP is the net GP from 200 mg dry sample after 24 h of incubation (GP₂₄) and after being corrected from its correction factor for the day-to-day variation in the activity of rumen fluid (ml) is expressed in ml/200 mg DM, and ash, CP and EE concentrations are expressed as g/kg DM.

Data analyses

To describe the dynamics of GP over time, the following Gompertz function (Schofield et al., Reference Schofield, Pitt and Pell1994) was chosen:

(7)$${\rm GP\ } = A{\rm \;exp\;}\left. {\left. {\left\{{-{\rm exp}\left[{1 + \displaystyle{b \over A}} \right.} \right.( {{\rm LAG}-t} ) } \right]} \right\}$$

where A is the theoretical maximum of GP, b is the maximum rate of GP (ml/h) that occurs at the point of inflection of the curve, LAG is the lag time (h) which is defined as the time-axis intercept of a tangent line at the point of inflection, and t is time (h). The parameters A, b and LAG were estimated by non-linear regression analysis (PROC NLIN; SAS 9.4, SAS Institute Inc., Cary, North Carolina, USA).

The fibre fractions, in vitro fibre digestibility, GP (i.e. 12, 24, 48 and 96 h of incubation), ME and NEL values were analysed using a mixed procedure (PROC MIXED) by SAS 9.4 (SAS Institute Inc.) according to:

(8)$$Y_{ijk} = \mu + \alpha _i + \beta _j + ( {\alpha \, \beta } ) _{ij} + R_k + e_{ijk}$$

where Y_ijk = the dependent variable; μ = the overall mean; α_i = the effect of hays of different quality (i.e. LQH, MQH and HQH); β_j = the inclusion levels of KL (i.e. 0, 50, 100 and 200 g/kg DM); (α β)_ij = the interaction of grass hay with different quality and inclusion levels of KL; R_k = the random effect of run; and e_ijk = the residual error. Linear effects of level were tested by orthogonal polynomial contrasts using the CONTRAST statement. Differences between means with P < 0.050 were accepted as statistically significant, and differences with 0.050 < P < 0.100 were considered to represent tendencies to significance.