Effect of Lipid Sources with Different Fatty Acid Profiles on Intake, Nutrient Digestion and Ruminal Fermentation of Feedlot Nellore Steers

Article information

Asian-Australas J Anim Sci. 2015;28(11):1583-1591
1Embrapa, Centro Nacional de Pesquisa de Gado de Leite, Juiz de Fora, MG 36038-330, Brazil
2Department of Animal Sciences, Instituto Nacional de Ciência e Tecnologia-Ciência Animal, Universidade Federal deViçosa, Viçosa, MG 36570-000, Brazil
*Corresponding Author: Giovani Fiorentini. Tel: +55-16-3209-2682, E-mail: giovanizoot@yahoo.com.br
Department of Animal Sciences, UNESP, Univ Estadual Paulista, Jaboticabal, SP 14884-900, Brazil
Received 2015 February 13; Revised 2015 April 07; Accepted 2015 May 08.

Abstract

The present study was conducted to determine the effect of lipid sources with different fatty acid profiles on nutrient digestion and ruminal fermentation. Ten rumen and duodenal fistulated Nellore steers (268 body weight±27 kg) were distributed in a duplicated 5×5 Latin square. Dietary treatments were as follows: without fat (WF), palm oil (PO), linseed oil (LO), protected fat (PF; Lactoplus), and whole soybeans (WS). The roughage feed was corn silage (600 g/kg on a dry matter [DM] basis) plus concentrate (400 g/kg on a DM basis). The higher intake of DM and organic matter (OM) (p<0.001) was found in animals on the diet with PF and WF (around 4.38 and 4.20 kg/d, respectively). Treatments with PO and LO decreased by around 10% the total digestibility of DM and OM (p<0.05). The addition of LO decreased by around 22.3% the neutral detergent fiber digestibility (p = 0.047) compared with other diets. The higher microbial protein synthesis was found in animals on the diet with LO and WS (33 g N/kg OM apparently digested in the rumen; p = 0.040). The highest C18:0 and linolenic acid intakes occurred in animals fed LO (p<0.001), and the highest intake of oleic (p = 0.002) and C16 acids (p = 0.022) occurred with the diets with LO and PF. Diet with PF decreased biohydrogenation extent (p = 0.05) of C18:1 n9,c, C18:2 n6,c, and total unsaturated fatty acids (UFA; around 20%, 7%, and 13%, respectively). The diet with PF and WF increased the concentration of NH3-N (p<0.001); however, the diet did not change volatile fatty acids (p>0.05), such as the molar percentage of acetate, propionate, butyrate and the acetate:propionate ratio. Treatments PO, LO and with WS decreased by around 50% the concentration of protozoa (p<0.001). Diets with some type of protection (PF and WS) decreased the effects of lipid on ruminal fermentation and presented similar outflow of benefit UFA as LO.

INTRODUCTION

The lipid addition in ruminant diets has been used to increase energy density, improve livestock system efficiency and to generate meat quality with human health benefits. However, the supplementation of lipids (e.g., high levels) may cause negative effects on ruminal fermentation, affecting fiber digestion and dry matter intake (DMI) (Manso et al., 2006). The lipid metabolism is highly variable in the rumen and total tract due to many factors, such as the nature and concentration of lipids in the diet, the type of chemical and/or physical treatments added to feeds, and the characteristics and the forages to concentrate ratio in the diet (Fiorentini et al., 2013).

Several types of lipids with different fatty acid composition can be used in ruminant diets (Duckett and Gillis, 2010), such as vegetable oils, oilseeds, and calcium salts of fatty acids (protected fat [PF]). Therefore, it is important to evaluate their effects on intake and digestion of nutrients to achieve desired animal production.

Our hypothesis is that sources with a saturated profile (palm oil [PO]) should demonstrate a lower impact on rumen fermentation and in the flow of unsaturated fatty acids (UFA) towards the duodenum. On the one hand, linseed oil (LO) addition should cause disorders on the ruminal fermentation due to defaunation and negative effects of free UFA on the bacterial membrane, but on the other hand, it could to enhance the flow of UFA to be absorbed in the duodenum. Lipid diets with some types of protection and with UFA profiles (soybean and PF) would be expected to increase the flow of fatty acid through the rumen without disturbing fermentation. Thus, the objective of this study was to evaluate these lipid sources with different fatty acid profiles on nutrient digestion and ruminal fermentation in Nellore steers.

MATERIALS AND METHODS

Animals and experimental feeds

The protocol used in this experiment was in accordance with the Brazilian College of Animal Experimentation (COBEA - Colégio Brasileiro de Experimentação Animal) guidelines and was approved by the Ethics, Bioethics, and Animal Welfare Committee (CEBEA - Comissão de Ética e Bem Estar Animal) of the FCAV–UNESP–Jaboticabal campus (protocol number 012799).

Ten Nellore steers (Bos taurus indicus; 15±2 months; 268 initial body weight±27 kg and 293 final body weight±27 kg), fitted with ruminal and duodenal cannulas, were used for the evaluation of the DMI and nutrients digestibility, protozoa quantification, ruminal pH, NH3-N, volatile fatty acids (VFA), and microbial protein synthesis in a duplicated 5×5 Latin square design experiment. The experimental period lasted 100 days, and it was divided into five periods of 20 days; the first 15 days comprised a period of adaptation to the diets, and the subsequent 5 days were used for data collection. During the adaptation period, animals were kept in partially covered individual pens equipped with a drinker and feed trough. In the sampling period, they were kept in metabolism cages with a wooden slotted floor, an individual drinker and feed trough, and boxes for a total collection of feces.

The diets were calculated as described by Fiorentini et al. (2014). Five concentrates were formulated: i) without additional fat (WF; 27.9 g/kg of ether extract [EE] in the total diet); ii) with PO derived from the palmaceae plant Orbignya oleifera, which has a lipid profile rich in lauric and myristic (medium-chain fatty acids); iii) with LO; iv) with whole soybeans (WS) – whole and unground; and v) PF (Lactoplus; Dalquim group, Itajaí, Santa Catarina, Brazil). PF (Lactoplus) is manufactured by a saponification process where fatty acids (based on soybean oil) react with calcium hydroxide. The diets LO and PO contained 45.0 g/kg of oil, the WS diet contained 138 g/kg of whole soybeans and the PF diet contained 51 g/kg of Lactoplus on dry matter (DM) basis. Thus, all of the diets with added lipids contained an average of 42 g of additional lipid per kg of DM.

The proportions of ingredients and the chemical composition of the experimental diets are presented in Table 1. The roughage was corn silage (600 g/kg on a DM basis and with the following composition: 369 g DM/kg, 71 g crude protein/kg DM, 477 g neutral detergent fiber (NDF)/kg DM, 23 g EE/kg DM, and 53 g lignin/kg DM) and concentrate (400 g/kg on a DM basis). The concentrates were mixed weekly to restrict oxidation and rancidity of ingredients. The lipid sources (PO, LO, PF, and WS) were incorporated into the remaining ingredients of the concentrate in a horizontal mixer for 15 min. The animals were fed with corn silage and the experimental concentrates once per day at 8:00 h. The concentrates and roughage from each animal were weighed individually and manually mixed in the troughs of each animal.

Composition of the experimental diets (g/kg DM)

Data collection and sampling procedures

Throughout the entire experimental period, the provided quantities were adjusted to allow a surplus of approximately 100 g/kg in relation to the total amount consumed on the previous day. Feed refusals were collected and weighed before feeding for the first 5 days of each experimental period, and subsamples were obtained and frozen at −20°C. Diet samples (roughage and concentrate) were collected weekly for each experimental period and frozen for subsequent chemical and nutrient evaluation. Samples of feces were collected for 5 days of each experimental period. Total fecal collection was used to determine the apparent digestibility. Representative 500 g of feces samples were collected at 8:00 h daily, weighed and homogenized. These samples were placed into plastic bags and frozen, and a composite sample was prepared for each animal based on the air-dry weight. Duodenal digest samples were collected as described by Fiorentini et al. (2013). Samples of feces and duodenal contents were dried in a forced-ventilation oven at 55°C for 72 h and ground in a mill with 1 mm mesh sieve.

Samples of feed offered, feed refusals, feces and duodenal digest were composited by treatment within period, dried at 55°C, and ground ground in a Wiley mill (Thomas Scientific, Swedesboro, NJ, USA) to pass a one mm screen. Samples of corn silage, concentrates, and feed refusals were analyzed for DM (934.01), MM (942.05), and acid EE (954.02) according to AOAC (1990). The EE contents in feces and duodenal digest were determined by extraction in ether (EE; 920.39). Nitrogen was determined using a LECO FP-528 nitrogen analyzer (LECO Co., St. Joseph, MI, USA). The NDF and acid detergent fiber were determined as described by Fiorentini et al. (2014). The gross energy content of feeds and refusals was determined using an adiabatic bomb calorimeter (PARR Instrument Company 6300, Moline, IL, USA). Chemical analyses were performed on each sample in duplicate, and when the coefficient of variation for the replicate analysis was more than 5%, the analysis was repeated.

Feed intake for each steer was calculated as the difference between the feed offered and refused during each period. Nutrient digestibilities were calculated by the following formula: [1–(output of nutrient/intake of nutrient)]×100. Indigestible NDF (iNDF) was used as an indicator of daily DM flows in the duodenum (Harvatine and Allen, 2006). This fiber was obtained via an in situ methodology after 240 hours (Casali et al., 2008) with incubated samples of feed offered, feed refusals, feces and ground duodenal digest (Wiley mill, 2 mm screen). The iNDF was analyzed using an Ankom Fiber Analyzer (Ankom Technology, Fairport, NY, USA). Duodenal DM flow was calculated according to the following equation (Fiorentini et al., 2013): Duodenal DM flow = [(fecal DM×g/kg iNDF in fecal DM)/g/kg iNDF in duodenal DM].

The extraction of fatty acids was conducted as described by Fiorentini et al. (2013). Fatty acids were quantified using a GC 20-10 gas chromatograph (Shimadzu Co., Kyoto, Japan; 100 m×0.20 mm i.d. with 0.02-μm film thickness; Supelco, Bellefonte, PA, USA) (Table 1). The biohydrogenation extent (BH) was calculated as described by Wu et al. (1991). BH = 100–100[(total duodenal digesta unsaturated 18C/total 18C in duodenal digesta)/(total unsaturated 18C intake/total 18C intake)].

To evaluate rumen fermentation parameters, rumen fluid samples (approximately 80 mL) were collected manually on the last day of each experimental period, both before supplying the diet (time zero) and 1, 2, 4, 6, 8, 10, 12, and 14 h after feeding. The samples were filtered through double-layer cotton fabric. Immediately after collection, the pH of rumen fluid was determined using a digital potentiometer (ORION 710A, Boston, MA, USA). A 2 mL aliquot of collected fluid was placed into a plastic bottle and frozen at −20°C for subsequent VFA analysis according to a method adapted from as described by Fiorentini et al. (2013). A 40 mL aliquot of rumen fluid was used for NH3-N analysis following the methodology adapted by Fenner (1965). On the last day of each experimental period ruminal samples (solid and liquid digest) were collected manually at 12:00 h for protozoa counts and analysis as described by Fiorentini et al. (2013).

Total urine was collected for 5 day each experimental period using funnel collectors attached to the animals. The funnel collector was connected to a polyethylene flexible tube, which directed the urine to containers containing 500 mL of H2SO4 (200 mL/L; volume/volume) to avoid loss of nitrogenous compounds. After each 24 h collection period, the total weight and volume of urine excreted was determined. A composite sample was made from the 5 sampling days. The composite sample was homogenized, and a 10 mL sub-sample was diluted with 40 mL of 0.018 mM H2SO4. Microbial protein synthesis was calculated via urinary total excretion of purine derivatives (PD; allantoin+uric acid), according to Pina et al. (2009).

Statistical analyses

Data of DMI, nutrients intake, digestibility, protozoa quantification, and microbial protein synthesis were analyzed as a double 5×5 Latin square using SAS PROC MIXED 2000 (SAS Institute Inc., Cary, NC, USA). Dietary treatments were considered fixed whereas steers and periods were random variables. The general mathematical model was represented as follows:

Yij=μ+Si+Ti+Pj+TPij+eij

where Yij is the dependent variable; μ is the overall mean; Si is the effect of steer i; Ti is the i th effect of the treatment or diet; Pj is the j th effect of the period; TPij is the effect of the interaction between treatment i and period j; and ɛij is the residual experimental error. In the statistical model, normally and independently distributed errors were assumed. Data of ruminal pH, NH3-N, and VFA were analyzed as double 5×5 Latin square using repeated measures according to the following model:

Yijkl=μ+Si+Ti+Pj+TPij+ɛijk+Hl+THkl+ωijkl

where Yij is the dependent variable; μ is the overall mean; Si is the effect of steer i; Ti is the i th effect of the treatment or diet; Pj is the j th effect of the period; TPij is the effect of the interaction between treatment i and period j; ɛijk is the whole plot error; Hl is the effect of the sampling time l; THkl is the interaction between treatment k and sampling time l, and ωijkl is the split plot error.

Differences between treatment means were determined by Tukey’s test. Significance was declared at p<0.05 and trends at 0.05<p<0.10.

RESULTS

The higher intake of DM and OM was found in animals fed PF and WF (p<0.001) (Table 2). Animals fed with WS had intermediate intake, whereas the diet PO had the lowest intake. The intake of DM and OM of animals fed with LO did not differ from PO and WS diets. The higher EE intake occurred in animals receiving PF (p<0.001). However, animals fed PO, showed intake similar to that of animals fed WF.

Effects of feeding supplemental lipid sources on nutrient intake and nutrient digestibility of Nellore steers

The treatments with PO and LO decreased total digestibility of DM (p = 0.021) and OM (p = 0.048). Animals fed WF diet had lower (p<0.001) EE digestibility than other diets. The addition of LO resulted in the lowest NDF digestibility (p = 0.047; 0.40 kg/kg), and the NDF digestibility was not different among the other diets. The diets PF and WF increased N intake (p = 0.010). The higher production of microbial N (p = 0.030) was in the animals fed WF, LO, and WS, whereas animals of the PO diet had the lowest production. The higher microbial protein synthesis was found in animals on the diet with LO and WS (p = 0.040) (Table 2).

Diets with PO increased intake of C8:0, C10:0, C12:0, and C14:0 as well as total SFA in relation to the other diets (p<0.001) (Table 3). The highest C18:0 and linolenic acid intake occurred in animals fed LO (p<0.001), and the highest intake of oleic (p = 0.002) and C16 acids (p = 0.022) occurred with the diets with LO and PF. Diets with PF and WS promoted greater intake of linoleic acid (C18:2 n6,c), total fatty acids and total UFA (p<0.05).

Effects of feeding supplemental lipid sources on intake and flow of the fatty acids of Nellore steers

The duodenal flow of C16:0, C18:0, oleic, elaidic (C18:1 n9,t), linoleic (C18:2 n6,c), linolenic, total SFA, and total UFA was affected by lipid sources (p<0.05) (Table 3). The highest flow of SFA and C18:0 was achieved with the diets containing LO, PF, and WS. The addition of LO increased (p = 0.02) duodenal flow of linolenic acid. The UFA flow was higher (p = 0.012) with the diet containing PF compared with the diets WF, PO, and WS. There were no differences for digestibility of the SFA, UFA, and total fatty acids (p>0.05) (Table 3). The treatment with PF had lower BH of C18:1 n9,c (p = 0.04), C18:2n6,c (p = 0.03), and total UFA (p = 0.044) (Table 3) than other diets.

The diet with PF and WF increased the concentration of NH3-N (p<0.001) (Table 4); however, the diet did not change in VFAs (p>0.05), such as the molar percentage of acetate (ACE), propionate (PROP), butyrate and the ACE:PROP ratio. There was a tendency (p = 0.06) to change ruminal pH values and total VFA (p = 0.092) with lipid diets. The number of protozoa of the genus Entodinium and total protozoa was affected by the lipid sources (p<0.001) (Table 5). Treatments PO, LO and with WS decreased by around 50% the concentration of protozoa (p<0.001).

Effects of feeding supplemental lipid sources on ruminal fermentation of Nellore steers

Effects of feeding supplemental lipid sources on the population of ciliated protozoa in the rumen of Nellore steers

DISCUSSION

In this study, we evaluated the influence of several lipid sources on ruminal digestion and fermentation as well as the extent of fatty acid biohydrogenation in the rumen. The decreased DMI in diets with LO, PO, and WS was in accordance with the results found in the literature, which show that the reduction in intake with the inclusion of fatty acids may be associated with reduced digestibility, especially in the fiber fraction of the diet (Wanapat et al., 2011). A negative effect on fiber digestibility was only observed in the diet with LO compared with the diets WF and those with PF. These observations may be linked to the number of double bonds in the fatty acid molecules and to the high availability of this source, which tends to reduce cellulolytic bacteria proportion (Yang et al., 2009). Although the DMI as a percentage of BW can be considered low for WF and PF, these values corroborated with Fiorentini et al. (2014), who worked with the same diets in a performance trial.

The intake and digestibility reduction in the PO diets rich in SFA with the same intensity as sources rich in UFA (LO and WS) was not expected, and these results differed from the discussions about the low disturbance of SFA supplementation on the ruminal environment, and consequently the reduction of negative effects on the fiber digestibility (Wanapat et al., 2011). According to Sullivan et al. (2004), diets containing more than 70 g/kg EE in the DM can impair feed degradation, especially if there is a high proportion of UFA, which had greater impact on rumen fermentation than SFA due to many factors, such as fiber coating, toxic effect to Gram-positive bacteria and protozoa (Soliva et al., 2004), and modifying hydrogen uptake by methanogens. It is likely that in addition to the SFA profiles of PO, other dietary factors, such as the low acceptance by animals and a possible toxicity effect of this lipid source, can be linked to the intake and digestibility reduction. Similarly, Otaru et al. (2011) verified a decreasing linear effect on DMI in goats fed diets with PO. Once the level of lipid addition is variable and dependent of the particular source of fatty acids used, type of animal, and method of lipid processing, there is no optimum level of lipid that can be added in the ruminant diet.

The increased EE digestibility in diets with lipid addition was consistent with the results of Manso et al. (2006). The higher digestibility coefficients in lipid-supplemented animals can be attributed the fact that non-fatty acids lipids in the diet (likely approximately 1% of DM) are relatively indigestible, and diluting this fraction (waxes, etc.) with more fatty acids increases the digestibility of the EE fraction.

The flow of fatty acids in the present study indicated the disappearance and modification of fatty acids in the rumen. According to Doreau and Ferlay (1994) and Schmidely et al. (2008), the negative balance of fatty acids (consumed/recovered in the duodenum) is frequent, especially in diets rich in lipids (more than 5% of fatty acids in the dietary DM). The disappearance of fatty acids in the rumen can be attributed to the following factors: i) absorption of fatty acids in the rumen as the amount of lipids in the diet increases; ii) catabolization of fatty acids in ketone bodies in the cells of the ruminal epithelium; and iii) oxidation of fatty acids by bacteria adherent to the rumen wall, which utilize oxygen from epithelial cells (Doreau and Ferlay, 1994). However, it is not possible to associate these effects with characteristics of the supplemental fat, e.g., protection or degree of saturation (Doreau and Ferlay, 1994). Thus, with the aim of evaluating ruminal biohydrogenation, Schmidely et al. (2008) worked in a meta-analysis (95 experiments and 303 treatments) and they estimated an average recovery of 75% of the fatty acids of the duodenum, thereby corroborating with current data. Sterk et al. (2012) reported low duodenal recovery of fatty acids in dairy cows diets with lipid addition of 55 to 65 g/kg DM.

The results of UFA and SFA flow indicated the effect of ruminal biohydrogenation, which is the passage of lipids of dietary and microbial origins into the duodenum (Jenkins, 1994). In fact, a greater quantity of C18:1 n9,t (elaidic acid), an intermediate product of biohydrogenation, was observed. These results are similar to those reported by Menezes et al. (2010) in crossbred steers (Charolais×Nellore) fed with 60% of corn silage and 40% of concentrate. The high ruminal outflow of SFA, especially C18:0, in animals fed diets with LO, PF, and WS may be explained by higher intake of oleic and linoleic acids in these treatments, which are SFA to C18:0 by rumen microorganisms through ruminal biohydrogenation (Duckett and Gillis, 2010). Both intake and presence of conjugated linoleic acid in duodenal digest were virtually nil in all treatments and these results corroborate with Menezes et al. (2010).

In an extensive review Doreau and Ferlay (1994) reported ruminal BH of linolenic averaged 92% (range, 85% to 100%) and BH of linoleic averaged 80% (range, 70% to 95%). The present ruminal BH was close to the range reported by Doreau and Ferlay (1994) for linolenic (range, 85.9% to 91.5%) and linoleic (range, 89.9% to 97.8%). As BH of oleic, the results found in this study were higher than those reported by Wu et al. (1991), who found values of the 44.2 in diets with 6% of PF. The BH total of UFA was lower in animals fed the diet with PF because calcium soaps in the rumen are not dissociated, thus delaying biohydrogenation by bacteria (Harvatine and Allen, 2006) and allowing UFA absorption in the duodenum and meat deposition. Our results were in accordance with previous literature reporting partial dissociation of calcium salts of soybean oil. Klusmeyer and Clark (1991) reported 50% protection with soybean against ruminal biohydrogenation calcium salts of soybean fatty acid. Similarly, Lundy et al. (2004) studied the addition of 2.75% soybean oil calcium salts in the diet of dairy cows, and they found biohydrogenation values of 77.9 and 92.2% for 18:1 (n9) and 18:2 (n3) acids, respectively. According to Jenkins and Bridges Jr. (2007), PF provide inconsistent results with limited ruminal protection. However, the PF could be advantageous over non-protected because of the higher amount of UFA in the rumen that can be harmful to microbial membranes and cause metabolic disorders, mainly in cellulolytic flora (Maia et al., 2007) or decreasing fiber digestibility.

We hypothesized that diet with the PF would have higher ruminal protection. This prediction was supported by our results, showing that PF has a variable dissociation in the rumen, which may increase BH total UFA. The PF utilized in this study originated from soybean oil rich in UFA. According to Jenkins and Bridges Jr. (2007), calcium salts with a high content of SFA are more efficiently protected than those with a low content of SFA. The dramatic reductions in the feed intake with LO, PO, and WS diets could have occurred due to a slower rate of passage and increase of ruminal feed retention time, which could also contribute to a higher BH total UFA. Nevertheless it is important to highlight the increase of linolenic acid flow in the LO diets with potential improvements in the UFA composition of the meat.

In the LO and PO diets with reduced OM content and possible reduction of feed fermentability, a lower concentration of VFA was expected (Harvatine and Allen, 2006). However, our results corroborated with studies in which a small or no effect on ruminal VFA concentration was observed with the addition of lipid sources to diets for ruminants (Fiorentini et al., 2013). Diets with vegetable oils cause higher variability on pH (Ivan et al., 2001), due to high levels of free UFA and are more susceptible to hydrolysis by rumen bacteria than diets containing calcium salts (Wu et al., 1991) and oilseeds (Ueda et al., 2003). On the other hand, these results may suggest that rumen ecology of Nellore steers could resist specific carbohydrate addition, or can increase the absorption of VFAs.

The decrease of ruminal NH3-N concentration with vegetable oil could have occurred due to protozoa action by reducing deaminating bacteria (Doreau and Ferlay, 1995). The higher NH3-N content in the WF and PF diets may be associated with a predominance of proteolytic protozoa that engulf the rumen bacteria and release NH3-N into the rumen environment (Doreau and Ferlay, 1995). In this scenario, even with increased nitrogen intake of the animals, the incorporation of NH3-N by rumen bacteria may be reduced, and the microbial protein synthesis may be compromised (Yang et al., 2009). The concentration of NH3-N in the rumen is a consequence of the balance between its production, absorption and utilization by microorganisms. The utilization efficiency of ammonia by the microorganisms for the microbial protein synthesis depends, among other factors, on the availability of energy in the rumen, thus withstanding greater microbial growth (Russell et al., 1992).

The reduction in the number of protozoa and the amount of NH3-N in the PO, LO, and WS diets may be linked to similar negative effects of UFA in the bacterial membrane (Maia et al., 2007). In spite of the significant level of saturation, PO reduced the population of protozoa and was not sufficient enough to increase the microbial protein synthesis. The decreased concentration of rumen NH3-N and the reduced number of rumen protozoa corroborated the results reported by Eugène et al. (2004) with defaunated animals.

The supply of vegetable oils frequently increases the microbial protein synthesis (Messana et al., 2013). However, the effect of vegetable oils on microbial synthesis is not mediated by an increase in the fermentable energy content of the rumen. Vegetable oils reduce predation due to the defaunation effect of the oil (Fiorentini et al., 2013). The reduction or elimination of protozoa could be associated with microbial protein synthesis, as protozoa engulf bacteria, but because of protozoa phagocytosis starch particles, this reduction would be associated with a possible reduction in the rumen ammonia concentration and a smaller and more variable pH (Ivan et al., 2001), therefore decreasing carbohydrate fermentation and maintaining a consistent pH.

CONCLUSION

Diets with some type of protection (PF and WS) decreased the effects of lipid on ruminal fermentation and presented similar outflow of benefit UFA as LO. However the PO diet impaired ruminal function parameters without contributing effectively in providing UFA into the duodenum of beef cattle.

ACKNOWLEDGMENTS

We thank the São Paulo Research Foundation (FAPESP) (grants #2009/ 51215-1; 2009/ 06472-6 and 2013/ 02418-2) and Bellman Nutrição Animal for providing financial support.

Notes

CONFLICT OF INTEREST

We certify that there is no conflict of interest with any financial organization regarding the material discussed in the manuscript.

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Article information Continued

Table 1

Composition of the experimental diets (g/kg DM)

Items Diets

WF PO LO PF WS
Ingredient
 Corn silage 600 600 600 600 600
 Ground corn 269 214 214 208 138
 Soybean meal 110 120 120 121 0.00
 Protected fat 0.00 0.00 0.00 51.0 0.00
 Whole soybean 0.00 0.00 0.00 0.00 250
 Linseed oil 0.00 0.00 45.0 0.00 0.00
 Palm oil 0.00 45.0 0.00 0.00 0.00
 Urea 9.00 9.00 9.00 9.00 0.00
 Mineral supplement1 12.0 12.0 12.0 12.0 12.0
Chemical composition
 Dry matter 562 569 568 563 563
 Organic matter 954 955 956 945 954
 Crude protein 160 160 161 164 164
 Ether extract 27.9 70.5 70.2 69.9 69.7
 Neutral detergent fiber 340 340 340 339 364
 Acid detergent fiber 195 196 198 196 220
 Metabolizable energy2 (MJ/kg) 10.9 10.7 10.8 12.2 11.9
 TDN3 719 841 840 845 838
Fatty acids (g/100 g of total fatty acids)
 C8:0 (caprylic) 0.00 0.90 0.00 0.00 0.00
 C10:0 (capric) 0.00 1.00 0.00 0.00 0.00
 C12:0 (lauric) 0.40 15.70 0.70 0.30 0.30
 C14:0 (myristic) 0.40 5.40 0.50 0.40 0.40
 C16:0 (palmitic) 19.7 16.6 18.7 19.0 17.5
 C16:1 (palmitoleic) 0.10 0.10 0.10 0.10 0.10
 C17:0 (margaric) 0.20 0.20 0.20 0.20 0.20
 C18:0 (stearic) 1.90 0.50 3.80 0.00 1.30
 C18:1 n9,c (oleic) 30.5 24.6 28.6 29.9 27.3
 C18:2 n6,c (linoleic) 43.3 31.8 36.3 45.9 46.3
 C18:3 n-3 (alpha linolenic) 2.80 2.80 11.20 4.40 4.10
 C20:0 (arachidic) 0.00 0.00 0.10 0.00 2.60

DM, dry matter; WF, without additional fat; PO, palm oil; LO, linseed oil; PF, protected fat (Lactoplus); WS, whole soybeans.

1

Composition of product expressed in g or mg per 100 g of supplement: calcium, 4.5 g; phosphorus, 1.2 g; magnesium, 4.6 g; sulfur, 1.4 g; sodium, 5.8 g; copper, 14 mg; manganese, 41 mg; zinc, 52.5 mg; iodine, 1 mg; cobalt, 0.8 mg; selenium, 0.3 mg; fluorine (maximun), 12 mg.

2

Metabolizable energy = total apparent digestibility of gross energy×0.82.

3

Total digestible nutrients as described by Fiorentini et al. (2014).

Table 2

Effects of feeding supplemental lipid sources on nutrient intake and nutrient digestibility of Nellore steers

Items Diets SEM p-value

WF PO LO PF WS
Intake (kg/d)
 Dry matter 4.50a 2.43c 3.09bc 4.26a 3.36b 0.32 <0.001
 Organic matter 4.32a 2.37c 3.00bc 4.07a 3.25b 0.31 <0.001
 Ether extract 0.09c 0.14c 0.23b 0.31a 0.21b 0.02 <0.001
 N intake 0.12a 0.08c 0.08c 0,12a 0,10b 0.08 0.010
 NDF 1.52 1.20 1.11 1.48 1.26 0.14 0.117
Total apparent digestibility (kg/kg)
 Dry matter 0.73a 0.65b 0.66b 0.75a 0.72a 0.02 0.021
 Organic matter 0.71a 0.64b 0.65b 0.74a 0.71a 0.02 0.048
 Ether extract 0.54b 0.80a 0.81a 0.83a 0.88a 0.06 <0.001
 NDF 0.51a 0.48a 0.40b 0.56a 0.51a 0.06 0.047
 OMDR (kg/d) 2.05 1.21 1.49 2.01 1.52 0.30 0.247
 Microbial N (g/d) 43.3a 19.7c 51.7a 34.0b 47.7a 6.70 0.030
Microbial protein synthesis (g N/kg OMDR) 21.1b 16.4b 34.6a 16.9b 31.4a 5.20 0.040

WF, without additional fat; PO, palm oil; LO, linseed oil; PF, protected fat (Lactoplus); WS, whole soybeans; SEM, standard error of the mean; NDF, neutral detergent fiber; OMDR, organic matter apparently digested in the rumen.

a,b,c

Means within a row with differing superscripts differ (Tukey’s test, p<0.05).

Table 3

Effects of feeding supplemental lipid sources on intake and flow of the fatty acids of Nellore steers

Items Diets SEM p-value

WF PO LO PF WS
Fatty acid intake (g/d)
 C8:0 (caprylic) 0.01b 4.08a 0.01b 0.01b 0.01b 0.21 <0.001
 C10:0 (capric) 0.01b 4.80a 0.01b 0.01b 0.01b 0.23 <0.001
 C12:0 (lauric) 0.16b 71.3a 1.16b 0.07b 0.27b 3.81 <0.001
 C14:0 (myristic) 0.28b 22.9a 0.54b 0.10b 0.20b 1.29 <0.001
 C16:0 (palmitic) 16.6b 26.5b 44.1a 33.4a 30.3b 5.88 0.022
 C18:0 (stearic) 0.72b 0.01b 13.10a 0.01b 2.03b 1.40 <0.001
 C18:1 n9,c (oleic) 21.1b 48.6b 73.7a 78.6a 56.8b 10.1 0.002
 C18:2 n6,c (linoleic) 87.1b 79.1b 99.5b 220a 201a 10.7 <0.001
 C18:3 n-3 (alpha linolenic) 1.35b 2.44b 52.1a 15.8b 5.62b 5.42 <0.001
 C20:0 (arachidic) 0.01b 0.01b 0.01b 0.01b 20.9a 0.48 <0.001
 Total intake 126c 260b 285b 348a 318a 23.40 <0.001
 SFA1 17.4c 130.2a 59.9b 33.7c 54.4b 8.75 <0.001
 UFA2 109c 130c 225b 315a 273a 17.30 <0.001
Flow to duodenum (g/d)
 C10:0 (capric) 0.71 4.27 1.99 3.66 3.36 1.90 0.590
 C12:0 (lauric) 1.71 7.20 3.99 7.19 2.79 1.87 0.080
 C14:0 (myristic) 0.71 0.31 1.02 1.38 0.35 0.40 0.230
 C16:0 (palmitic) 25.5b 21.2b 35.7b 67.3a 32.4b 9.88 0.011
 C18:0 (stearic) 96.3b 60.0b 138a 129a 165a 28.50 0.042
 C18:1 n9,c (oleic) 10.4ab 5.96b 22.7ab 34.5a 13.2ab 4.02 0.011
 C18:1 n9,t (elaidic) 3.77b 2.17b 12.90ab 21.50a 1.75b 6.51 0.022
 C18:2 n6,c (linoleic) 4.10ab 1.48b 2.33ab 7.58ab 9.32a 2.01 0.020
 C18:3 n3 (alpha linolenic) 0.24c 0.15c 1.17a 0.68b 0.65b 0.29 0.292
 C20:0 (arachidic) 1.08 0.75 0.82 5.72 1.92 1.99 0.041
 SFA1 126b 94.6b 183a 217a 206a 35.10 0.043
 UFA2 18.8b 9.70b 39.9ab 65.2a 25.5b 9.91 0.012
Total digestibility (kg/kg)
 Total fatty acids 0.86 0.89 0.84 0.89 0.91 0.04 0.620
 SFA1 0.70 0.88 0.80 0.62 0.81 0.11 0.351
 UFA2 0.87 0.88 0.86 0.93 0.93 0.04 0.292
Ruminal biohydrogenation extent (%)
 C18:1 n9,c (oleic)3 73.9a 73.0a 71.0a 58.6b 72.7a 5.34 0.040
 C18:2 n6,c (linoleic)3 94.9a 96.5a 97.8a 89.9b 94.1a 1.58 0.030
 C18:3 n3 (alpha linolenic)3 85.9 86.7 89.8 91.4 91.5 6.56 0.110
 BH total UFA4 87.3a 89.1a 84.6a 76.7b 89.1a 2.68 0.044

WF, without additional fat; PO, palm oil; LO, linseed oil; PF, protected fat (Lactoplus); WS, whole soybeans; SEM, standard error of the mean; SFA, saturated fatty acids; UFA, unsaturated fatty acids.

1

SFA = C4:0; C6:0; C8:0; C10:0; C12:0; C13:0iso; C13:0ant; C14:0iso; C14:0; C15:0iso; C15:0ant; C14:1c9; C15:0; C16:0iso; C16:0; C17:0iso; C17:0; C18:0; C20:0; C22:0; C24:0.

2

UFA = C16:1c9; C17:1; C18:1t6; C18:1t9; C18:1t10; C18:1t11; C18:1t12; C18:1c9; C18:1c11; C18:1c12; C18:1c13; C18:1t16; C18:1c15; C18:2t11c15; C18:2c9c12; C18:3; C18:2c9t11; C20:1; C24:1; C20:3; C20:4; C20:5; C22:1; C22:2; C22:5; C22:6; C24:1.

3

Individual 18-C unsaturated fatty acid biohydrogenation, % =−100 {100×(individual 18-C UFA/total 18-C in duodenal digesta)/(individual 18-C UFA/total 18-C intake)}.

4

Biohydrogenation of total unsaturated C18 fatty acids = 100–100×{(TDDUC18/TC18DD)}/{(TUC18I/TC18I)}; where, TDDUC18 = total duodenal digesta unsaturated C18; TC18DD = total C18 in duodenal digesta; TUC18I = total unsaturated C18 intake; TC18I = total C18 intake.

a,b,c

Means within a row with differing superscripts differ (Tukey’s test, p<0.05).

Table 4

Effects of feeding supplemental lipid sources on ruminal fermentation of Nellore steers

Items Diets SEM p-value


WF PO LO PF WS Diet Time Diet×time
NH3-N (mg/dL) 16.6a 7.09b 7.33b 13.9a 9.28b 1.39 <0.001 <0.001 0.102
pH 6.21 6.37 6.51 6.24 6.32 0.08 0.065 <0.001 0.567
Total VFA (mmol/L) 90.3 72.6 78.3 92.6 79.5 8.21 0.092 0.012 0.329
VFAs (%)
 ACE 66.9 65.2 64.3 67.0 63.5 2.10 0.631 <0.001 0.197
 PROP 20.9 23.1 25.1 21.1 25.5 1.93 0.198 <0.001 0.263
 Butyrate 12.2 11.7 10.6 11.9 11.0 0.83 0.568 <0.001 0.556
 ACE:PROP ratio 3.20 2.82 2.56 3.17 2.49 0.29 0.325 <0.001 0.681

WF, without additional fat; PO, palm oil; LO, linseed oil; PF, protected fat (Lactoplus); WS, whole soybeans; SEM, standard error of the mean; VFA, volatile fatty acid; ACE, acetate; PROP, propionate.

a,b

Means within a row with differing superscripts differ (Tukey’s test, p<0.05).

Table 5

Effects of feeding supplemental lipid sources on the population of ciliated protozoa in the rumen of Nellore steers

Diets SEM p-value

WF PO LO PF WS
Protozoa (n∘×105/mL)
 Entodinium 25.6a 7.90b 2.21b 22.3a 2.24b 4.31 <0.001
 Epidinium 0.03 0.00 0.00 0.00 0.00 0.02 0.476
 Diplodininae 0.70 0.02 0.02 1.28 0.01 0.12 0.342
 Total 26.3a 7.92b 2.23b 23.6a 2.25b 4.39 <0.001

WF, without additional fat; PO, palm oil; LO, linseed oil; PF, protected fat (Lactoplus); WS, whole soybeans; SEM, standard error of the mean.

a,b

Means within a row with differing superscripts differ (Tukey’s test, p<0.05).