Soluble Non-ammonia Nitrogen in Ruminal and Omasal Digesta of Korean Native Steers Supplemented with Soluble Proteins

Article information

Asian-Australas J Anim Sci. 2012;25(9):1269-1275
1National Institute of Animal Science, RDA, 441-706, Korea.
2Department of Animal Science, Chonbuk National University, Jeonju, 561-756, Korea.
*Corresponding Author: Chang Weon Choi. Tel: +82-53-850-6721, Fax: +82-53-850-6729, E-mail: changchoi@daegu.ac.kr
Department of Animal Resources, Institute of Life and Environment, Daegu University, Jillyang, Gyeongsan 712-714, Korea
Received 2012 June 08; Accepted 2012 June 20; Revised 2012 July 03.

Abstract

An experiment was conducted to study the effect of soluble protein supplements on concentration of soluble non-ammonia nitrogen (SNAN) in the liquid phase of ruminal (RD) and omasal digesta (OD) of Korean native steers, and to investigate diurnal pattern in SNAN concentration in RD and OD. Three ruminally cannulated Korean native steers in a 3×3 Latin square design consumed a basal diet of rice straw and corn-based concentrate (control), and that supplemented (kg/d DM basis) with intact casein (0.24; IC) or acid hydrolyzed casein (0.46; AHC). Ruminal digesta was sampled using a vacuum pump, whereas OD was collected using an omasal sampling system at 2.0 h intervals after a morning feeding. The SNAN fractions (free amino acid (AA), peptide and soluble protein) in RD and OD were assessed using the ninhydrin assay. Concentrations of free AA and total SNAN in RD were significantly (p<0.05) lower than those in OD. Although free AA concentration was relatively high, mean peptide was quantitatively the most important fraction of total SNAN in both RD and OD, indicating that degradation of peptide to AA rather than hydrolysis of soluble protein to peptide or deamination may be the most limiting step in rumen proteolysis of Korean native steers. Diurnal variation in peptide concentration in OD for the soluble protein supplemented diets during the feeding cycle peaked 2 h post-feeding and decreased thereafter whereas that for the control was relatively constant during the entire feeding cycle. Diurnal variation in peptide concentration was rather similar between RD and OD.

INTRODUCTION

Studies of feed evaluation using the nylon bag method were performed based on an assumption that the ‘a-fraction’, which is rapidly degradable nitrogen (N) in the rumen, of feed was infinitely degraded and consequently that only insoluble feed N could escape the rumen (Ørskov and McDonald, 1979; Madsen et al., 1995; Volden and Harstad, 1995). Many in vivo studies, however, reported that a substantial soluble non-ammonia N (SNAN) concentration may escape the rumen of dairy cows (Chen et al., 1987a, 1987b; Robinson and McQueen, 1994), which is inconsistent with the assumption of the nylon bag studies. For example, Choi et al. (2002b) reported that approximately 110 mg/L of SNAN was detected in omasal digesta of dairy cows supplemented with skimmed milk powder, which completely disappeared from nylon bags during the zero h washing procedure (Choi, 2002). Chen et al. (1987a) also reported that an increase in crude protein (CP) of diets (14.5 to 17.5% DM basis) did not affect flow of peptide and soluble protein in RD. In addition, Broderick and Wallace (1988) showed a peak of ruminal peptide concentration immediately after feeding when casein was fed.

The SNAN data in the studies described above (Chen et al., 1987a, 1987b; Broderick and Wallace, 1988; Robinson and McQueen, 1994) were achieved from mainly dairy cows fed relatively high CP. It may be in general accepted that a considerable amount of SNAN from dairy cows fed high CP diets, even soluble protein and non-protein N, can escape ruminal degradation (Choi et al., 2002b). Besides, the SNAN escaping ruminal degradation may increase milk production including milk protein synthesis (Choi et al., 2002b). However, few SNAN studies using beef cattle fed relatively low CP diets compared to dairy cows were available. Quantification of SNAN from beef cattle may be important because Swanson et al. (2002) and Richard et al. (2003) reported that abomasal infusion of glucose (and/or starch) with soluble protein increased glucose (and/or starch) utilization in the small intestine of beef steers compared with starch infusion alone. Thus, the more SNAN escaping the rumen may increase intramuscular fat of beef cattle through high glucose utilization because Smith and Crouse (1984) as reported that glucose was primarily utilized for intramuscular fat synthesis compared to other carbon sources, i.e. acetate, lactate, etc.

The present study, therefore, aimed to study the effect of soluble protein supplements on the concentration of SNAN in ruminal (RD) and omasal digesta (OD) of Korean native beef cattle fed rice straw and corn-based concentrate supplemented with different soluble proteins and to investigate diurnal patterns in the SNAN concentration in RD and OD.

MATERIALS AND METHODS

Animals and diets

Three Korean native beef steers weighing on an average 779 (SE±21.1) kg and fitted with 100 mm i.d. ruminal cannula were used in a 3×3 Latin square experiment. The animals were housed individually in 3×3.2 m pens with concrete floors in a temperature and light controlled (23°C and 16 h of light/8 h of dark, respectively) room with water and a trace-mineralized salt block available throughout the experiments. The steers were weighed before each period. They were provided with two equal meals daily at 09:00 and 17:00 h.

The steers were offered rice straw and corn-based concentrate ad libitum during an adaptation period, and then the DMI was restricted to 90% of the ad libitum intake. A basal diet (% DM) consisted of rice straw (31.3) and concentrate (68.8) (control). Concentrate (% DM) contained corn (50.8), wheat bran (38.0), soybean meal (3.0), rapeseed meal (2.0), molasses (2.0), limestone (1.5), salt (0.4) and vitamin and minerals (0.3). Part of the basal diet was replaced (kg/d) by one of two protein supplements as follows: intact casein (0.24) (IC; 100% protein), or acid hydrolyzed casein (0.46) (AHC; 80% AA+20% peptide).

Sampling procedures and chemical analysis

Each period lasted 21 d. Feed intake was recorded daily. Representative samples of feeds were collected on d 15 to 21, pooled, subsampled, dried and ground through a 1-mm screen with a Wiley mill (Thomas Scientific, Model 4, NJ, USA) for analysis. Feed DM concentration was determined using a forced-air oven for 18 h at 105°C. Approximate analysis of experimental feeds was performed according to AOAC (1990). To estimate SNAN fractions in digesta, RD and OD were collected at 0, 2, 4, 6, and 8 h post-feeding on d 21. RD was sampled from the rumen via the ruminal cannula, and OD was collected from the omasal canal by means of a plastic tube (14 mm i.d.) connected to a pump according to procedures outlined by Huhtanen et al. (1997), with the exceptions as follows: i) larger sampling tube (14 vs 9.5 mm i.d.), ii) solenoid valves instead of a three way ball valve to control vacuum and pressure phases in a pump and iii) a 0.5 kg weight inserted into the abomasum two secure the sampling device in the omasum. Approximately 300 ml samples of RD and OD were filtered through four layers of cheesecloth and saturated HgCl2 added to prevent microbial activity. Filtrates of RD and OD were centrifuged at 1,000×g for 10 min at 4°C, and the supernatant was decanted into a fresh tube followed by high-speed centrifugation (10,000×g, 30 min, 4°C) to remove small particles and rumen microbes. The supernatant was precipitated with trichloroacetic acid (TCA) (final concentration 5% w/v), placed in ice overnight and high-speed centrifuged (10,000×g, 30 min, 4°C). Different N fractions (free AA, peptide and soluble protein) of SNAN in the liquid phase of RD and OD were assessed using a ninhydrin assay. Details of SNAN fractions analyses have previously been described by Choi (2002). In brief, SNAN within RD and OD was fractionated as follows: i) free AA: estimated from the supernatant without acid-hydrolysis, ii) peptide: estimated from hydrolysed supernatant (6 M HCl, 24 h, 110°C) minus free AA and iii) soluble protein: estimated from hydrolysis of TCA-precipitate, respectively. All SNAN fractions were corrected for ammonia N except for soluble protein because TCA-precipitate was assumed to contain negligible amounts of ammonia N.

Statistical analysis

Data on intake of dietary ingredients were fitted using the MIXED procedure of SAS (2002) according to the following statistical model:

Yijk=μ+Ai+Pj+Dk+eijk

where A is a random effect of animal, and P and D are the fixed effects of period and diet, respectively.

Data on SNAN fractions of RD and OD determined at each sampling interval were fitted using the MIXED procedure of SAS (2002) for repeated measures according to the following statistical model:

Yijkl=μ+Ai+Pj+Dk+eijk+Tl+(A×T)il+(P×T)jl+(D×T)kl+eijkl

where T is a fixed effect of time after feeding, and A×T, P×T and D×T are animal by time, period by time and diet by time interactions, respectively. In the repeated measures models, animal, animal by time interaction and error terms (eijk defined as between unit error and eijkl as within unit error) are assumed to be multivariate normally distributed random effects with AR (1) covariance structure. Orthogonal contrasts used in post-ANOVA comparisons were as follows; i) effect of casein supplements (control vs IC+AHC), ii) effect of casein types (IC vs AHC), iii) effect of intact casein (control vs IC) and iv) effect of acid hydrolyzed casein (control vs AHC), respectively.

RESULTS AND DISCUSSION

Feeds

The chemical composition of experimental feeds is given in Table 1. Experimental animals consumed rice straw and concentrates as planned (Table 2). Soluble protein supplements had no effect (p>0.05) on total DMI, but increased CP intake (p = 0.006).

Chemical composition of experimental feeds

Intake of dietary ingredients

Metabolism of SNAN

Concentration of SNAN fractions in the liquid phase of RD and OD is given in Table 3. Soluble protein supplements did not affect (p>0.05) free AA concentration in RD. These results contrast with those of Choi et al. (2002b), in which dietary soluble protein (skimmed milk powder and wet distiller’s soluble) increased free AA in RD of dairy cows fed grass silage based diets. Compared with control, IC tended (p = 0.09) to increase free AA concentration in OD. Relatively high concentration of free AA in both RD and OD is consistent with a previous study (Choi et al., 2002b). However, Choi et al. (2002a) reported a relatively low concentration of free AA (mean 15.9 mg N/l) in OD. Also, Nolan (1993) reviewed that free AA concentration was very low even immediately after feeding.

Effect of soluble protein supplements on concentration (mg/L) of soluble non-ammonia nitrogen fractions in ruminal (RD) and omasal digesta (OD) of Korean native steers

Soluble protein supplements statistically increased peptide concentration in RD (p = 0.02) and OD (p = 0.002), whereas the protein types did not affect (p>0.05) peptide N. This observation is rather similar to that of Choi et al. (2002b), where soluble protein tended to increase peptide N despite lack of significance. In the study of Choi et al. (2002b), peptide N was not affected by soluble protein types. Absolute value of peptide in RD in the present study (77.3 mg/L) was relatively lower than published values (82 to 111 mg/L) (Chen et al., 1987a; Robinson and McQueen, 1994; Robinson et al., 1998). This may be because the previous studies have analysed free AA and peptide together, whereas we analysed net peptide. If free AA and peptide are pooled together, the sum (124.1 mg/L) in the present study is slightly higher than the previous value cited above. Despite relatively high free AA concentration, peptide N in RD and OD averaging 77.3 and 81.6 mg/L, respectively, was quantitatively the most important N in SNAN fractions. This result clearly supports our suggestion that degradation of peptide to AA may be the rate-limiting step in protein degradation in the rumen (Choi et al., 2002a, 2002b; Oh et al., 2008). Thus, the previous observation that hydrolysis of protein to peptide or deamination may be the rate-limiting step in rumen proteolysis (Wright and Hungate, 1967; Chen et al., 1987b; Van Straalen and Tamminga, 1990) is not valid.

Neither soluble protein supplements nor their types affect (p>0.05) soluble protein concentration in either RD or OD. Mean concentration of soluble protein in RD (19.8 mg/L) and OD (18.9) are in good agreement with reported values (12 to 37 mg/L) by Robinson and McQueen (1994), Robinson et al. (1998) and Oh et al. (2008). Inconsistent with the present result, Choi et al. (2002b) reported extremely low soluble protein concentration in RD and OD (1.0 and 1.2 mg/L, respectively) when different proteins were supplemented to dairy cows.

A considerable amount of SNAN fractions including peptide and free AA in OD determined from beef cattle in the present study may be important because soluble protein infusing into the abomasum increased glucose and/or starch utilization in the small intestine of beef steers (Richard et al., 2002; Swanson et al., 2002). Smith and Crouse (1984) observed that glucose was primarily utilized for bovine intramuscular fat synthesis rather than acetate, lactate, etc. In addition, starch digestion in the small intestine is more energetically efficient than its fermentation in the rumen (Richards et al., 2003). Taniguchi et al. (1995) also suggested that protein supply can improve starch digestion in the small intestine of beef cattle. Further studies on relationship between omasal SNAN concentration and intramuscular fat synthesis including starch utilization in the small intestine of beef cattle is required.

Rumen vs omasum in SNAN

In the present study, free AA in OD was significantly (p<0.05) higher than that in RD, supporting a similar result of Kim et al. (2009), where Korean native steers supplemented with protein had higher free AA in OD than that in RD (24.9 vs 20.1 mg N/L). In the present study, no statistical significance (p>0.05) in peptide concentration between RD and OD was observed. This is not in agreement with previous study (Choi et al., 2002b), where peptide in OD was considerably higher than that in RD. The discrepancy between the present and the previous studies is unclear; however this may be related to the soluble protein and CP levels in experimental diets. In other words, Choi et al. (2002b) used grass silage as a basal diet including high soluble N and relatively high CP (approximately 15.3 to 17.6%) for dairy cows in lactation. In the present study, intact and acid hydrolyzed casein as protein supplements were mainly in the forms of soluble protein and AA including 20% peptide, respectively, thus peptide concentrations did not clearly differ between RD and OD. In addition, the steers in the present study consumed relatively low CP (11.4 to 14.4%, Table 2). Similar to the peptide results, soluble protein concentration between RD and OD did not statistically differ (p>0.05).

Diurnal variation in SNAN

Diurnal variation in mean concentration of SNAN fractions in RD are shown in Figure 1. Dietary soluble protein supplements did not affect (p>0.05) diurnal variation in free AA concentration. Diurnal variation in free AA concentration for all groups was relatively constant with no clear peaks during an entire feeding cycle. This result may support a previous observation that ruminal free AA concentration was relatively low even immediately post-feeding (Nolan, 1993). Broderick and Wallace (1988) also reported that diurnal variation in free AA was relatively constant during a feeding cycle when sheep consumed 67% ryegrass hay and 33% concentrate with ovalbumin supplementation. Mean concentration of peptide in RD appeared to be highest at 2 h post-feeding and declined thereafter. Compared with control, mean peptide concentration for IC and AHC was numerically higher during the entire feeding cycle. Diurnal variation in ruminal peptide concentration in RD is consistent with previous studies (Robinson and McQueen, 1994; Robinson et al., 1998; Oh et al., 2008) in which the diurnal variation peaked immediately after feeding and declined thereafter. In addition, Broderick and Wallace (1988) reported that peptide reached a maximum immediately after feeding when casein was supplemented, even though diurnal variation in peptide concentration was rather constant throughout a feeding cycle in sheep fed hay and corn-based concentrate. As with the ruminal free AA pattern, soluble protein concentration was relatively constant throughout the feeding period. In contrast with the present results, previous studies showed clear peaks of soluble protein concentration at 1 to 3 h post-feeding (Robinson and McQueen, 1994; Robinson et al., 1998; Oh et al., 2008).

Figure 1

Diurnal pattern in concentration of free amino acids (AA) (A), peptide (B) and soluble protein (C) in the liquid phase of ruminal digesta (RD) during a feeding cycle as influenced by soluble protein supplements (Markers indicate no supplement (♦), intact casein (■) and acid hydrolyzed casein (▲), respectively).

Unlike the ruminal free AA, when soluble protein was supplemented diurnal variation in omasal free AA concentration was the highest at 2 h after feeding, declined till 4 h and then remained relatively constant throughout the remainder of the feeding cycle. This result is similar to a previous result reported by Oh et al. (2008) in which dietary protein supplements showed clear peaks in omasal free AA concentration immediately post-feeding. In contrast, rapeseed meal supplementation did not show clear peaks of omasal free AA concentration in dairy cows fed grass based diets (Choi, 2007). Diurnal variation in peptide concentration in OD being similar with that in RD (Figures 1 and 2) and appeared to be highest at 2 h post feeding and declined thereafter except for the control. This result is consistent with previous results (Choi et al., 2002c; Oh et al., 2008) where various protein supplements showed a peptide peak immediately post-feeding. The present peptide pattern may support a previous observation (Oh et al., 2008) that dietary soluble proteins were rapidly degraded to peptides in the rumen shortly after consumption. Protein supplements did not affect diurnal variation in soluble protein concentration entering into the omasum. Soluble protein concentration was relatively constant throughout the feeding period. Consistent with the present results, some studies showed no clear peaks of soluble protein concentration during the entire feeding cycle (Choi and Choi, 2003; Oh et al., 2008).

Figure 2

Diurnal pattern in concentration of free amino acids (AA) (A), peptide (B) and soluble protein (C) in the liquid phase of omasal digesta (OD) during a feeding cycle as influenced by soluble protein supplements (Markers indicate no supplement (♦), intact casein (■) and acid hydrolyzed casein (▲), respectively).

ACKNOWLEDGEMENTS

This study was supported by Cooperation Research Project (No. PJ007800062012), Rural Development Administration, Republic of Korea.

References

AOAC. 1990. Official methods of analysis 15th ed Association of Official Analytical Chemists Washington, DC, USA:
Broderick GA, Wallace RJ. 1988;Effects of dietary nitrogen source on concentrations of ammonia, free amino acids and fluorescamine-reactive peptides in the sheep rumen. J Anim Sci 66:2233–2238.
Chen G, Sniffen CJ, Russell JB. 1987a;Concentration and estimated flow of peptides from the rumen of dairy cattle: Effects of protein quantity, protein solubility, and feeding frequency. J Dairy Sci 70:983–992.
Chen G, Russell JB, Sniffen CJ. 1987b;A procedure for measuring peptides in rumen fluid and evidence that peptide uptake can be a rate-limiting step in ruminal protein degradation. J Dairy Sci 70:1211–1219.
Choi CW. 2002. Assessment of the flow of soluble dietary non-ammonia nitrogen escaping degradation in the rumen of dairy cows fed grass silage based diets. Doctoral dissertation University of Helsinki. Department of Animal Science; Viikki. Finland:
Choi CW. 2007;Diurnal patterns in the flow of escapable soluble non-ammonia nitrogen fractions in omasal digesta as influenced by barley and rapeseed meal supplementation in cows fed grass silage based diet. J Anim Sci Technol 49:341–350.
Choi CW, Choi CB. 2003;Flow of soluble non-ammonia nitrogen in the liquid phase of digesta entering the omasum of dairy cows given grass silage based diets. Asian-Aust J Anim Sci 16:1460–1468.
Choi CW, Ahvenjärvi S, Vanhatalo A, Toivonen V, Huhtanen P. 2002a;Quantitation of the flow of soluble non-ammonia nitrogen entering the omasal canal of dairy cows fed grass silage based diets. Anim Feed Sci Technol 96:203–220.
Choi CW, Vanhatalo A, Ahvenjärvi S, Huhtanen P. 2002b;Effects of several protein supplements on flow of soluble non-ammonia nitrogen from the forestomach and milk production in dairy cows. Anim Feed Sci Technol 102:15–33.
Choi CW, Vanhatalo A, Huhtanen P. 2002c;Concentration and estimated flow of soluble non-ammonia nitrogen entering the omasum of dairy cows as influenced by different protein supplements. Agric Food Sci Finl 11:79–91.
Huhtanen P, Brotz PG, Satter LD. 1997;Omasal sampling technique for assessing fermentative digestion in the forestomach of dairy cows. J Anim Sci 75:1380–1392.
Kim JH, Oh YK, Kim KH, Choi CW, Hong SK, Seol YJ, Kim DH, Ahn GC, Song MK, Park KK. 2009;Effects of protein supply from soyhulls and wheat bran on ruminal metabolism, nutrient digestion and ruminal and omasal concentrations of soluble non-ammonia nitrogen of steers. Asian-Aust J Anim Sci 22:1267–1278.
Madsen J, Hvelplund T, Weisbjerg MR, Bertilsson J, Olsson I, Spörndly R, Harstad OM, Volden H, Tuori M, Varvikko T, Huhtanen P, Olafsson BL. 1995;The AAT/PBV protein evaluation system for ruminants. A revision. Norw J Agric Sci (Suppl)19:1–37.
Nolan JV. 1993. Nitrogen kinetics. Quantitative aspects of ruminant digestion and metabolism In : Forbes JM, France J, eds. CAB International Wallingford. Oxon, UK: p. 123–143.
Oh YK, Kim JH, Kim KH, Choi CW, Kang SW, Nam IS, Kim DH, Song MK, Kim CW, Park KK. 2008;Effects of level and degradability of dietary protein on ruminal fermentation and concentrations of soluble non-ammonia nitrogen ruminal and omasal digesta of Hanwoo steers. Asian-Aust J Anim Sci 21:392–403.
Ørskov ER, McDonald P. 1979;The estimation of protein degradability in the rumen from incubation measurements weighted according to rate passage. J Agric Sci (Camb) 92:499–503.
Richards CJ, Branco AF, Bohnert DW, Huntington GB, Macari M, Harmon DL. 2002;Intestinal starch disappearance in steers abomasally infused with starch and protein. J Anim Sci 80:3361–3368.
Richards CJ, Swanson KC, Paton SJ, Harmon DL, Huntington GB. 2003;Pancreatic exocrine secretion in steers infused postruminally with casein and cornstarch. J Anim Sci 81:1051–1056.
Robinson PH, McQueen RE. 1994;Influence of supplemental protein source and feeding frequency on rumen fermentation and performance in dairy cows. J Dairy Sci 77:1340–1353.
Robinson PH, Veira DM, Ivan M. 1998;Influence of supplemental protein quality on rumen fermentation, rumen microbial yield, forestomach digestion, and intestinal amino acid flow in late lactation Holstein cows. Can J Anim Sci 78:95–105.
SAS. 2002. Statistical analysis systems. User’s guide: Statistics Version 9.1 Editionth ed. 2002. SAS Inst, Inc. Cary, NC, USA:
Smith SB, Crouse JD. 1984;Relative contributions of acetate, lactate and glucose to lipogenesis in bovine intramuscular and subcutaneous adipose tissue. J Nutr 114:792–800.
Swanson KC, Richards CJ, Harmon DL. 2002;Influence of abomasal infusion of glucose or partially hydrolyzed starch on pancreatic exocrine secretion in beef steers. J Anim Sci 80:1112–1116.
Taniguchi K, Huntington GB, Glenn BP. 1995;Net nutrient flux by visceral tissues of beef steers given abomasal and ruminal infusions of casein and starch. J Anim Sci 73:236–249.
Van Straalen WM, Tamminga S. 1990. Protein degradation of ruminant diets. Feedstuff evaluation 1 Livestock Feedingstuffs Composition In : Wiseman J, Cole DJA, eds. Butterworths. London, UK: p. 55–72.
Volden H, Harstad OM. 1995;Effect of rumen incubation on the true indigestibility of feed protein in the digestive tract determined by nylon bag techniques. Acta Agric Scand, Sect A, Animal Sci 45:106–115.
Wright DE, Hungate RE. 1967;Amino acid concentration in rumen fluid. Appl Environ Microbiol 15:148–151.

Article information Continued

Figure 1

Diurnal pattern in concentration of free amino acids (AA) (A), peptide (B) and soluble protein (C) in the liquid phase of ruminal digesta (RD) during a feeding cycle as influenced by soluble protein supplements (Markers indicate no supplement (♦), intact casein (■) and acid hydrolyzed casein (▲), respectively).

Figure 2

Diurnal pattern in concentration of free amino acids (AA) (A), peptide (B) and soluble protein (C) in the liquid phase of omasal digesta (OD) during a feeding cycle as influenced by soluble protein supplements (Markers indicate no supplement (♦), intact casein (■) and acid hydrolyzed casein (▲), respectively).

Table 1

Chemical composition of experimental feeds

Rice straw Concentrate Intact casein Acid hydrolysates
Composition, % Dry matter (DM)
 DM (%) 93.56 88.13 92.94 92.28
 Crude protein 4.45 14.66 87.11 49.13
 Ether extract 1.34 3.74 3.68 0.10
 Crude fiber 37.04 5.86 1.00 0.37
 Crude ash 11.90 5.12 5.24 44.93

The water and vitamin and mineral block were available at all times.

Table 2

Intake of dietary ingredients

Item Diet1
SEM2 Statistical significance3
Control IC AHC C1 C2 C3 C4
Dry matter intake (DMI, kg/d)
 Rice straw 1.78 1.80 1.68 0.068 0.48 0.14 0.70 0.19
 Concentrate 3.91 3.63 3.47 0.084 0.07 0.29 0.14 0.06
 Intact casein 0.24
 Acid hydrolyzed casein 0.46
 Total DMI 5.68 5.67 5.61 0.121 0.29 0.21 0.77 0.17
 Crude protein 0.65 0.82 0.81 0.019 0.006 0.369 0.007 0.008
1

Control = Rice straw+concentrate; IC = Rice straw+concentrate+intact casein; AHC = Rice straw+concentrate+acid hydrolyzed casein.

2

SEM = Standard error of the mean.

3

C1 = Effect of casein supplements; C2 = Effect of casein types; C3 = Effect of intact casein; C4 = Effect of acid hydrolyzed casein.

Table 3

Effect of soluble protein supplements on concentration (mg/L) of soluble non-ammonia nitrogen fractions in ruminal (RD) and omasal digesta (OD) of Korean native steers

Item Diet1
SEM2 Statistical significance3
Control IC AHC C1 C2 C3 C4 Site
Free amino acids (AA)
 RD 47.3 45.1 47.9 1.25 0.44 0.10 0.15 0.61 46.8a
 OD 48.2 64.2 61.9 6.06 0.07 0.79 0.09 0.14 58.1b
Peptide
 RD 63.7 85.7 82.5 5.23 0.02 0.67 0.02 0.04 77.3
 OD 65.6 82.9 96.4 4.28 0.002 0.06 0.02 <0.001 81.6
Soluble protein
 RD 20.1 18.5 20.7 1.23 0.73 0.28 0.40 0.78 19.8
 OD 18.8 19.2 18.7 0.88 0.85 0.62 0.68 0.93 18.9
SNAN
 RD 131.2 149.3 151.1 5.31 0.03 0.82 0.06 0.05 143.9c
 OD 132.6 166.3 177.0 5.85 0.004 0.25 0.01 0.004 158.6d
1

Control = Rice straw+concentrate; IC = Rice straw+concentrate+intact casein; AHC = Rice straw+concentrate+acid hydrolyzed casein.

2

SEM = Standard error of the mean.

3

C1 = Effect of casein supplements; C2 = Effect of casein types; C3 = Effect of intact casein; C4 = Effect of acid hydrolyzed casein.