Effects of Dietary Protein Levels for Gestating Gilts on Reproductive Performance, Blood Metabolites and Milk Composition

Article information

Asian-Australas J Anim Sci. 2014;27(1):83-92
School of Agricultural Biotechnology, Seoul National University, 1 Gwanak-ro, Gwanak-gu, Seoul 151-921, Korea
*Corresponding Author: Y. Y. Kim. Tel: +82-2-880-4801, Fax: +82-2-878-5839, E-mail: yooykim@snu.ac.kr
1Animal and Food Sciences, University of Kentucky, Lexington, USA.
2Department of Food and Nutrition, Jangan University, Hwaseong, Gyeonggi-do, Korea.
Received 2013 June 28; Revised 2013 September 12; Accepted 2013 August 13.

Abstract

This experiment was conducted to evaluate the effects of dietary CP levels in gestation under equal lysine content on reproductive performance, blood metabolites and milk composition of gilts. A total of 25 gilts (F1, Yorkshire×Landrace) were allotted to 4 dietary treatments at breeding in a completely randomized design, and fed 1 of 4 experimental diets containing different CP levels (11%, 13%, 15%, or 17%) at 2.0 kg/d throughout the gestation. Body weight of gilts at 24 h postpartum tended to increase linearly (p = 0.09) as dietary CP level increased. In lactation, backfat thickness, ADFI, litter size and weaning to estrus interval (WEI) did not differ among dietary treatments. There were linear increases in litter and piglet weight at 21 d of lactation (p<0.05) and weight gain of litter (p<0.01) and piglet (p<0.05) throughout the lactation as dietary CP level increased. Plasma urea nitrogen levels of gilts in gestation and at 24 h postpartum were linearly elevated as dietary CP level increased (p<0.05). Free fatty acid (FFA) levels in plasma of gestating gilts increased as dietary CP level increased up to 15%, and then decreased with quadratic effects (15 d, p<0.01; 90 d, p<0.05), and a quadratic trend (70 d, p = 0.06). There were no differences in plasma FFA, glucose levels and milk composition in lactation. These results indicate that increasing dietary CP level under equal lysine content in gestation increases BW of gilts and litter performance but does not affect litter size and milk composition. Feeding over 13% CP diet for gestating gilts could be recommended to improve litter growth.

INTRODUCTION

Protein and amino acids play crucial roles in reproductive performance of sows (Kim et al., 2009). Pettigrew and Yang (1997) reported that an adequate supply of protein and amino acids during gestation allowed sows to maintain their productivity, and that high body protein content of sows could maximize milk production and subsequent reproductive performance. NRC (1998) recommended 12.9% CP in gestation diets for gilts (average 125 kg of BW at breeding). However, modern gilts, genetically improved to have large litter and high milk production, require more nutrients to carry on normal reproductive cycle and body maturation (Boyd et al., 2000).

In previous studies, restricted dietary protein for gestating gilts did not affect litter size and litter birth weight but caused detrimental effects on litter weight gain although sufficient protein was provided during lactation (Baker et al., 1970; Kusina et al., 1999b). On the other hand, high dietary protein for gestating gilts increased litter weight and weight gain (Mahan, 1998), and elevated milk yield as well (Kusina et al., 1999b).

Recently, Zhang et al. (2011) reported sows fed gestation diets containing higher lysine levels (0.65 to 0.75%) than NRC (1998) recommendation under the same content of CP showed improvements in reproductive performance and litter growth, indicating lysine content in the gestation diets need to be increased. However, there is no evidence for the effect of dietary CP levels under high lysine content in gestation for gilts. Even though lysine has been considered the first-limiting amino acid in corn-soybean meal diets for sows in gestation and lactation, the other essential amino acids play important roles in the efficiency of protein utilization by gestating sows (Kim et al., 2009). Increased supply of dietary CP in gestation could allow gilts to consume adequate amino acids to maximize reproductive performance and ensure body development. Therefore, the objective of this experiment was to evaluate the effect of dietary CP levels for gestating gilts on reproductive performance including milk composition and their progeny’s appearance.

MATERIALS AND METHODS

Animal management, housing and experimental diets

At 180 d of age and approximately 105 kg BW, a total of 30 gilts (F1, Yorkshire×Landrace, Darby, Icheon, Korea) were housed in environmentally controlled pens (2.5×3.5 m2) with 3 gilts per pen. The gilts were given ad libitum access to feed and water through a feeder and a water cup nipple. At 220 d of age, the gilts were moved into individual gestation stalls (2.40×0.64 m2) and fed a total of 2 kg/d of a commercial gestation diet twice daily. After estrus check at approximately 240 d of age and 140 kg of BW, the gilts were artificially inseminated (Darby AI center, Choongju, Korea) by 3 times at 12 h interval. Then, 25 gilts were selected and allotted to 1 of 4 dietary treatments in a completely randomized design. Four experimental diets containing different CP levels of 11%, 13%, 15%, and 17% were provided to the gilts during gestation. Each diet in gestation contained 3,265 kcal of ME/kg, 0.74% of total lysine and the assigned content of CP, respectively. The protein content was adjusted with corn, soybean meal and corn gluten meal to meet each assigned CP level of treatments. A lactation diet containing 3,269 kcal of ME/kg, and 1.08% of total lysine was provided after farrowing regardless of gestation treatments. All nutrients met or exceeded NRC (1998) nutrient requirement estimates. The formula and chemical composition of experimental diets are presented in Table 1.

The formula and chemical composition of experimental diets in gestation and lactation (as-fed basis)1

Gestating gilts were housed in individual stalls (2.40×0.64 m2) which were installed on a concrete floor in a temperature-controlled room with automatic fans and individually fed a total of 2.0 kg/d divided equally between two meals fed at 08:00 and 16:00 during the entire gestation period. Pregnancy was confirmed on 28 d of gestation via ultrasound (Eagle scan, Dong Jin BLS Co, LTD., Gwangju, Korea). After 110 d of gestation, all gilts were moved into farrowing crates (2.5×1.8 m2) and housed until weaning.

After parturition, the lactation diet was provided and gradually increased from 1.0 kg/d by 0.5 kg/d until 5 d postpartum with a free access to water. From 5 d postpartum, feed and water were provided ad libitum to primiparous sows. Within 24 h postpartum, Fe-dextran (150 ppm) injection, ear notching, needle teeth clipping and tail docking were practiced to each piglet. Piglets were cross-fostered across treatments within 3 d after birth to balance suckling intensity across sows with equalization of litter size, and thus to minimize any impact of initial litter size potentially affecting litter growth.

Data collection

Body weight and backfat thickness of gilts were measured at mating, 110 d of gestation, 24 h postpartum and 21 d of lactation. An ultrasound device (Lean-meter, Renco Corp., Minneapolis, US) was used for measuring backfat thickness at P2 position (mean value from both sides of the last rib and 65 mm away from the backbone). The numbers of total born, born alive, stillborn and mummified piglets were recorded within 24 h postpartum and the number of pigs was recorded after cross-fostering and at 21 d of lactation. Lactation feed intake was recorded weekly. Piglet weight was recorded at 24 h postpartum, after cross-fostering and at 21 d of lactation. Litter weight was calculated by summing the individual piglet weights. Weaning to estrus interval (WEI) was determined by monitoring for estrus from 3 to 10 d after weaning.

Sample collections and analysis

For the initial, blood samples were randomly taken from 11 gilts immediately before mating. Colostrum, milk and blood samples were collected from 5 sows with 10 to 12 piglets from each treatment and 5 piglets (1/sow) were used to collect blood. Blood samples were collected from gilts through jugular vein into EDTA tubes at 15, 35, 70, 90, and 110 d of gestation as well as 24 h and 21 d postpartum and from nursing piglets through anterior vena cava at 24 h and 21 d after birth. Blood samples were centrifuged at 1,700 g at 4°C for 15 min (Eppendorf centrifuge 5810R, Hamburg, Germany) to separate plasma. Colostrum and milk were collected from the first and second teats at 24 h and 21 d postpartum after an intravascular injection with 5 IU oxytocin (Komi oxytocin inj. Komipharm International Co., Ltd., Siheung, Korea) in the ear. All samples were stored at −20°C until analysis.

Diets were analyzed for CP by the Kjedahl method (984.13; AOAC, 2005). Proximate analysis of colostrum and milk was conducted using Milkoscan FT 120 (FOSS Electric, Sungnam, Korea). Plasma urea nitrogen (PUN) level was analyzed using a blood analyzer (Ciba-Corning model, Express Plus, Ciba Corning Diagnostics Co., Massachusetts, US). Plasma free fatty acid (FFA) levels were determined using Wako FFA C Kit (Wako Chemical, Osaka, Japan), and plasma glucose level was detected by an enzymatic kit (Glucose Hexokinase Kit, Bayer, Pennsylvania, US). The amino acid contents in colostrum, milk and diets were determined by ion-exchange chromatography (Amino Acid Analyzer L-8900, Hitachi, Tokyo, Japan) with post-column derivatization with ninhydrin. Performic acid was used in oxidizing amino acids and neutralized with sodium citrate dihydrate, and then hydrolyzed with 6 N HCl for 22 h at 110°C to be liberated from the protein. Amino acids were quantified with the internal standard method (amino acid mixture standard solution Type H, Wako Chemical, Osaka, Japan; L-cysteic acid, Tokyo Chemical Industry, Tokyo, Japan; DL-methionine sulfone, Sigma, Missouri, US) by measuring the absorption of reaction products with ninhydrin at 570 nm.

Statistical analysis

Data were analyzed by ANOVA for a completely randomized design using the GLM procedure of SAS (SAS Institute, 2004). Least squares means were calculated for each independent variable. Orthogonal polynomial contrasts were used to determine linear and quadratic effects by increasing dietary CP levels in gestation for all measurements of sows and piglets. Individual sows and their litters were used as the experimental unit. Blood plasma data were analyzed by repeated measures ANOVA. Alpha level used for the determination of significance for all analysis was 0.05 and tendency for all analysis was p>0.05 and p<0.10.

RESULTS

One sow was removed from 11% CP treatment due to severe delivery problem and her piglets were cross-fostered to balance the number of suckling piglets. Body weight and backfat thickness of gilts in gestation and lactation did not differ among dietary treatments (Table 2). However, BW at 24 h postpartum (p = 0.09) tended to be linearly increased by increasing dietary CP level. No differences were observed in ADFI and WEI in lactating sows among dietary treatments.

Effect of CP levels in gestation diets on BW, backfat thickness and weaning to estrus interval of gilts in gestation and lactation

No significant differences were found in litter size as well as litter and piglet weight at birth and after cross-fostering (Table 3). Linear increases on weight of litter and piglet (p<0.05) at 21 d of lactation and weight gain of litter (p<0.01) and piglet (p<0.05) were observed as dietary CP level increased.

Effect of CP levels in gestation diets on litter size and litter performance of primiparous sows

Plasma urea nitrogen level was linearly increased at 15, 35, 70, 90 (p<0.01) and 110 d (p<0.05) of gestation by increasing dietary CP level in gestation (Table 4), and gestating gilts fed 17% CP diet had the highest PUN level at 15, 35, 70, 90, and 110 d of gestation among dietary treatments. Plasma FFA levels were increased as dietary CP level increased up to 15%, then decreased with quadratic effects at 15 d (p<0.01) and 90 d (p<0.05), and a quadratic trend at 70 d (p = 0.06) of gestation. In plasma glucose level, there were a quadratic effect at 15 d (p<0.05) and a similar trend at 70 d (p = 0.06) of gestation. Plasma values in gestation were changed over time (p<0.01). Plasma levels of FFA and glucose were the highest at 110 d of gestation whereas PUN level was the lowest. There was a day×treatment interaction (p<0.05) in PUN level in which the difference of PUN levels from 11% to 17% CP treatments decreased at 110 d of gestation. During lactation (Table 5), a linear increase at 24 h postpartum (p<0.01) but a trend of linear decrease at 21 d of lactation (p = 0.10) were observed in PUN levels by increasing dietary CP level. Quadratic trends in plasma FFA level at 24 h postpartum (p = 0.07) and in plasma glucose at 21 d of lactation (p = 0.10) were observed by increasing dietary CP level. Plasma glucose and PUN levels of lactating sows were changed over time (p<0.01). The PUN level of sows increased but plasma glucose level decreased from 24 h postpartum to 21 d of lactation. There was a day×treatment interaction (p<0.01) in PUN level in which a linear increase in PUN levels at 24 h postpartum by increasing dietary CP levels was not detected at 21 d of lactation. No differences were detected on PUN and plasma glucose levels of nursing pigs in lactation. Plasma glucose (p<0.05) and PUN (p<0.01) levels in nursing pigs were changed over time and PUN level decreased but plasma glucose level increased from birth to 21 d of lactation.

Effect of CP levels in gestation diets on blood profiles of gilts in gestation1

Effect of CP levels in gestation diets on blood profiles of primiparous sows and their progeny in lactation1

Dietary CP levels in gestation did not affect colostrum and milk compositions (Table 6). Arginine content in colostrum (Table 7) showed a linear decrease (p = 0.06) as dietary CP level increased. Histidine (p<0.05) content decreased as dietary CP level increased up to 15%, then increased with a quadratic effect. Isoleucine (p<0.05) and lysine content tended to decrease as dietary CP level increased up to 13% (p = 0.09), then increased with quadratic effects. With a quadratic effect (p<0.05) the highest cysteine concentration was observed when gilts were fed the 15% CP diet in gestation than the other treatment diets. Glycine (p<0.05) content increased as dietary CP level increased up to 13%. Quadratic increases were observed with trends in serine (p = 0.06) and tyrosine (p = 0.08) contents as dietary CP level increased up to 15%. In milk (Table 8), linear decreases were observed in arginine (p<0.01), methionine (p<0.01) and cysteine (p<0.05) content by increasing dietary CP level. Glutamic acid (p<0.05) and proline (p = 0.07) content increased linearly by increasing CP levels.

Effect of CP levels in gestation diets on milk composition of primiparous sows1

Effect of CP levels in gestation diets on amino acid composition (g/100 g milk protein) in colostrum of primiparous sows1

Effect of CP levels in gestation diets on amino acid composition (g/100 g milk protein) in milk of primiparous sows at 21 d of lactation1

DISCUSSION

Effect of high protein intake in gestation has been reported to increase milk production and BW at farrowing, and improve subsequent reproductive performance of gilts (Belstra et al., 1998; Mahan, 1998; Kusina et al., 1999b). In the current study, BW of gilts at farrowing tended to be linearly increased by increasing CP level. Previous studies consistently reported high protein intake in gestation increased sow BW at farrowing, and weight gain in gestation (Mahan and Mangan, 1975; Heo et al., 2008; Zhang et al., 2011), indicating that increasing protein intake in gestation could increase body reserves with protein deposition (Mahan, 1998; Kusina et al., 1999b). Similarly, Jones and Maxwell (1982) reported a quadratic increase of daily weight gain of gilts by increasing protein intake in gestation even though protein intake did not affect BW of gilts. Therefore, the increase of protein intake in gestation could increase body protein reserves of gestating gilts through the slight increase of BW.

When gestating gilts were fed 11% CP diet, the lowest BW change was observed numerically in overall lactation among dietary treatments. Heo et al. (2008) reported a high protein intake in gestation and lactation reduced sow BW loss in lactation. However, in this study, the sows consumed the same lactation diet during lactation. Thus, this observation might be associated with ADFI of sows and litter growth in lactation. Even though ADFI of sows in lactation did not differ by dietary CP levels, the lowest litter performance was observed when gilts were fed 11% CP diet in gestation. Therefore, it is likely that low piglet growth in 11% CP treatment with similar feed intake may result in lower maternal BW loss compared with the other treatments.

Litter size and WEI were not affected by dietary treatments in the current study, which agreed with previous studies. Tydlitat et al. (2008) reported increasing protein level in gestation diets did not affect total number born but resulted in decreased total number of born alive and increased stillborn piglet. Shields et al. (1985) also reported similar results in which litter size was not affected by dietary protein level in gestation. Concerning WEI, Greenhalgh et al. (1977) observed a longer WEI in sows fed low protein diet for gestation (9% CP) and lactation (13% CP) compared with those fed high protein diet for gestation (11% or 13% CP) and lactation (17% CP). The WEI could be delayed due to low plasma insulin concentration in lactation, and high glucose but low FFA concentrations in plasma of weaning sows (Armstrong et al., 1986) as well as high maternal protein loss during lactation (Clowes et al., 2003), resulting in a reduced subsequent reproductive performance. In this study, plasma glucose and FFA concentrations of sows at weaning had no considerable differences among dietary treatments, indicating that dietary protein level did not affect WEI.

In the current study, piglet birth weight was not affected by dietary CP level, which agreed with Tydlitat et al. (2008) who reported mean birth weight of piglets did not differ by dietary protein levels in gestation. Even though low CP level (11%) in gestation diet showed no negative effects on litter and piglet birth weight in this study, litter growth was the lowest among dietary treatments, which agreed with the previous work of Mahan (1998) who reported high dietary CP levels with high feed intake in gestation increased litter weight and gain, more in primiparous sows than old sows. Based on the results of the current study, 11% CP level in the gestation diet under equal lysine content was not enough to maximize litter growth which may be attributed to lack of the other essential amino acids available in the diet compared with the other diets. Insufficient amino acid content in gestation diets caused failure to normal litter growth in lactation, because of inadequate body protein reserves to produce milk, limitation of mammary gland development and damage to fetuses during gestation (Kusina et al., 1999a). Therefore, high CP level had a positive influence on litter growth but 11% CP level in gestation diet was not sufficient for gestating gilts to maximize piglet growth.

The PUN level in gestation increased linearly by increasing CP level, which agreed with Kusina et al. (1999b) who reported that PUN level increased by increasing protein content in gestation diets. The PUN is a good indicator of protein utilization in animal body and low concentration of blood urea may be derived from reduced availability of ammonia caused by enhanced protein synthesis and reduced amino acid oxidation (Wu and Morris, 1998). In this study, with equal lysine content 11% CP diet showed the lowest PUN level in gestation, meaning that protein utilization was the highest among dietary treatments. Additionally, the reduced patterns of PUN levels as gestation progressed indicated protein utilization increased in late gestation. The PUN is affected by several factors such as genders, feeding methods, protein level and quality (Eggum, 1970). A partial replacement of protein sources by animal- or plant-based protein ingredients had no effect on PUN concentration in pigs (Sun et al., 2009) whereas protein level in the diet had a positive correlation with PUN concentration in pigs (Eggum, 1970). In this study, dietary protein level was adjusted by cereal grains (soybean meal and corn gluten meal), and gilts fed high protein diets in gestation showed high PUN level throughout gestation with linear increases by dietary protein levels, which agreed with these previous studies. On the other hand, plasma values of sows at 21 d of lactation were not significantly different among dietary treatments because lactating sows were fed the same diet ad libitum and lactation feed intake was not different among dietary treatments. In addition, PUN and plasma glucose level of suckling pigs were not affected by protein levels in gestation diets, which resulted from similar milk composition among treatments. These results indicated that there were no major effects on blood profiles of lactating sows and their progeny by increasing protein level in gestation diets, which was in agreement with Heo et al. (2008).

In this study, plasma FFA levels were the highest at 110 d of gestation and the gestating gilts fed 15% CP diet showed the highest plasma FFA level in gestation with quadratic responses. The FFA levels were represented for satisfying energy demands and reflected fat mobilization from body reserves (Chilliard, 1993). Belstra et al. (1998) reported that plasma FFA level in gestation reached a peak level when energy needs for sows were the greatest, and that it reflected body fat mobilization. These results might indicate the energetic requirement of sows during gestation was the highest in late gestation and increased as dietary CP level increased up to 15% for mammary gland development, and thereby those sows could have high litter growth in lactation. However, there are a few evidences about the effect of dietary protein level on blood FFA of sows, thus further study is needed to demonstrate this effect clearly.

In the current study, dietary CP levels in gestation diets did not affect proximate composition of colostrum and milk. In contrast, it has been reported that high protein intake in gestation increased protein content in colostrum (Heo et al., 2008; Zhang et al., 2011). In this study, quadratic effects on histidine, isoleucine, cysteine, glycine, and with tendencies lysine, serine and tyrosine content in colostrum and linear effects on arginine, methionine, cysteine, glutamic acid, and with a tendency proline in milk were observed as dietary CP level increased in gestation but the results were variable by dietary CP level. Elliott et al. (1971) reported that milk composition was not affected by dietary factors, especially protein but essential amino acids in colostrum of sows fed low CP diet were the lowest and increased by increasing dietary protein level. Consequently, the litter growth was linearly increased by increasing dietary CP levels. Based on these results, increased litter growth by increasing CP levels in gestation diets might be explained by increase of milk yield, not improvement of milk composition. Further study is needed to clearly demonstrate a possible correlation between protein level in gestation and milk production and quality.

IMPLICATIONS

Several effects of increasing protein levels in gestation diets were observed in reproductive performance and blood parameters even though lysine content was similar between dietary treatments: i) High CP content in gestation diets for gilts had positive effects on sow body reserves. ii) Increased dietary CP level in gestation for gilts improved litter growth during lactation but did not affect litter size and litter birth weight. iii) The PUN level in gestation increased as dietary CP level increased but plasma FFA levels were the highest when 15% CP diet was provided to gestating gilts. Consequently, above 13% CP may be recommended for gestating gilts to maximize piglet growth.

ACKNOWLEDGEMENT

This study was supported by Rural Development Administration (RDA; Project No. PJ009226), Republic of Korea.

References

2005. Official methods of analysis 18th editionth ed. Association of Official Analytical Chemists. Washington DC, US:
Armstrong JD, Britt JH, Kraeling RR. 1986;Effect of restriction of energy during lactation on body condition, energy metabolism, endocrine changes and reproductive performance in primiparous sows. J Anim Sci 63:1915–1925.
Baker DH, Becker DE, Jensen AH, Harman BG. 1970;Reproductive performance and progeny development in swine as influenced by protein restriction during various portions of gestation. J Anim Sci 31:526–530.
Belstra BA, Richert BT, Frank JW. 1998. Effect of gestation dietary crude protein level on the gestation and lactation performance of primiparous sows. Purdue University 1998 Swine Day Reports p. 60–64.
Boyd RD, Touchette KJ, Castro GC, Johnston ME, Lee KU, Han K. 2000;Recent advances in amino acid and energy nutrition of prolific sows. Asian-Aus J Anim Sci 13:1638–1652.
Chilliard Y. 1993;Dietary fat and adipose tissue metabolism in ruminants, pigs, and rodents: A review. J Dairy Sci 76:3897–3931.
Clowes EJ, Aherne FX, Foxcroft GR, Barocos VE. 2003;Selective protein loss in lactating sows is associated with reduced litter growth and ovarian function. J Anim Sci 81:753–764.
Eggum BO. 1970;Blood urea measurement as a technique for assessing protein quality. Br J Nutr 24:983–988.
Elliott RF, Vander Noot GW, Gilbreath RL, Fisher H. 1971;Effect of dietary protein level on composition changes in sow colostrum and milk. J Anim Sci 32:1128–1137.
Greenhalgh JFD, Elsley FWH, Grubb DA, Lightfoot AL, Saul DW, Smith P, Walker N, Williams D, Yeo ML. 1977;Coordinated trials on the protein requirements of sows. 1. A comparison of four levels of dietary protein in gestation and two in lactation. Anim Prod 24:307–321.
Heo S, Yang YX, Jin Z, Park MS, Yang BK, Chae BJ. 2008;Effects of dietary energy and lysine intake during late gestation and lactation on blood metabolites, hormones, milk composition and reproductive performance in primiparous sows. Can J Anim Sci 88:247–255.
Jones RD, Maxwell CV. 1982;Growth, reproductive performance and nitrogen balance of gilts as affected by protein intake and stage of gestation. J Anim Sci 55:848–856.
Kim SW, Hurley WL, Wu G, Ji F. 2009;Ideal amino acid balance for sows during gestation and lactation. J Anim Sci 87:E123–E132.
Kusina J, Pettigrew JE, Sower AF, Hathaway MR, White ME, Crooker BA. 1999a;Effect of protein intake during gestation on mammary development of primiparous sows. J Anim Sci 77:925–930.
Kusina J, Pettigrew JE, Sower AF, White ME, Crooker BA, Hathaway MR. 1999b;Effect of protein intake during gestation and lactation on the lactational performance of primiparous sows. J Anim Sci 77:931–941.
Mahan DC, Mangan LT. 1975;Evaluation of various protein sequences on the nutritional carry-over from gestation to lactation with first-litter sows. J Nutr 105:1291–1298.
Mahan DC. 1998;Relationship of gestation protein and feed intake level over a five-parity period using a high-producing sow genotype. J Anim Sci 76:533–541.
National Research Council. 1998. Nutrient requirements of swine 10th Edth ed. National Academy Press. Washington, DC:
Pettigrew JE, Yang H. 1997;Protein nutrition of gestating sows. J Anim Sci 75:2723–2730.
SAS Institute Inc. 2004. SAS/STAT user’s guide SAS Institute Inc. Cary, NC:
Shields RG Jr, Mahan DC, Maxson PF. 1985;Effect of dietary gestation and lactation protein levels on reproductive performance and body composition of first-litter female swine. J Anim Sci 60:179–189.
Sun Z, Ma Q, Li Z, Ji C. 2009;Effect of partial substitution of dietary spray-dried porcine plasma or fishmeal with soybean and shrimp protein hydrolysate on growth performance, nutrient digestibility and serum biochemical parameters of weaning piglets. Asian-Aust J Anim Sci 22:1032–1037.
Tydlitat D, Vinkler A, Czanderlova L. 2008;Influence of crude protein intake on the duration of delivery and litter size in sows. Acta Vet Brno 77:25–30.
Valros A, Rundgren M, Špinka M, Saloniemi H, Rydhmer L, Hultén F, Uvnäs-Moberg K, Tománek M, Krejcí P, Algers B. 2003;Metabolic state of the sow, nursing behaviour and milk production. Livest Prod Sci 79:155–167.
Wu G, Morris SM Jr. 1998;Arginine metabolism: Nitric oxide and beyond. Biochem J 336:1–17.
Zhang RF, Hu Q, Li PF, Xue LF, Piao XS, Li DF. 2011;Effects of lysine intake during middle to late gestation (day 30 to 110) on reproductive performance, colostrum composition, blood metabolites and hormones of multiparous sows. Asian-Aust J Anim Sci 24:1142–1147.

Article information Continued

Table 1

The formula and chemical composition of experimental diets in gestation and lactation (as-fed basis)1

Item Protein level in gestation (%) Lactation

11.44 12.93 15.04 17.13
Ingredients (%)
 Corn 82.16 77.25 72.33 67.40 67.42
 Soybean meal (45% CP) 8.86 13.20 17.52 21.80 24.62
 Wheat bran 3.50 3.50 3.50 3.50 2.50
 Corn gluten meal 0.00 0.85 1.70 2.55 0.00
 Sugar molasses 0.50 0.50 0.50 0.50 1.05
 Soybean oil 0.90 1.00 1.10 1.20 1.00
 L-lysine HCl 0.40 0.27 0.13 0.00 0.38
 DL-methionine 0.07 0.02 0.00 0.00 0.00
 Dicalcium phosphate 2.62 2.30 1.96 1.64 1.50
 Limestone 0.28 0.42 0.60 0.76 0.78
 Vitamin premix2 0.20 0.20 0.20 0.20 0.20
 Mineral premix3 0.10 0.10 0.10 0.10 0.10
 Salt 0.26 0.24 0.21 0.20 0.30
 Choline chloride-50 0.15 0.15 0.15 0.15 0.15
Analyzed chemical composition (%)
 CP 11.44 12.93 15.04 17.13
 Essential amino acids
 Arg 0.58 0.80 0.87 1.06
 His 0.26 0.36 0.36 0.42
 Ile 0.39 0.53 0.57 0.69
 Leu 0.97 1.31 1.42 1.69
 Lys 0.67 0.84 0.76 0.82
 Met 0.27 0.32 0.25 0.30
 Phe 0.46 0.64 0.69 0.83
 Thr 0.38 0.54 0.55 0.66
 Val 0.55 0.74 0.77 0.91
 Non-essential amino acids
 Ala 0.58 0.78 0.82 0.96
 Asp 0.87 1.25 1.32 1.61
 Cys 0.22 0.23 0.25 0.28
 Glu 2.01 2.75 2.84 3.42
 Gly 0.41 0.57 0.59 0.71
 Pro 0.67 0.90 0.91 1.07
 Ser 0.48 0.69 0.70 0.83
 Tyr 0.34 0.43 0.49 0.60
1

Daily feed provision in gestation was 2.0 kg/d and lactation feed was provided ad libitum.

2

Provided per kg of diet: vitamin A, 10,000 IU; vitamin D3, 1,500 IU; vitamin E, 35 IU; vitamin K, 3 mg; vitamin B2, 4 mg; vitamin B6, 3 mg; vitamin B12, 15 μg; pantothenic acid, 10 mg; biotin, 50 μg; niacin, 20 mg; folic acid 500 μg.

3

Provided per kg of diet: Fe, 75 mg from FeSO4; Mn, 20 mg from MnSO4; Zn, 30 mg from ZnSO4; Cu, 55 mg from CuSO4; Se, 100 μg from Na2SeO3; Co, 250 mg from CoSO4; I, 250 μg from Ca(IO3)2.

Table 2

Effect of CP levels in gestation diets on BW, backfat thickness and weaning to estrus interval of gilts in gestation and lactation

Item Protein level in gestation (%) SEM1 p-value


11.44 12.93 15.04 17.13 Linear Quadratic
No. of sows 5 7 6 6
BW (kg)
 At mating 140.5 139.1 139.7 139.8 3.00 0.902 0.813
 110 d of gestation 201.9 207.1 204.0 205.3 3.77 0.694 0.610
 Gestation gain (d 0 to 110) 61.4 67.9 64.3 65.5 2.08 0.377 0.213
 24 h postpartum 179.6 189.3 186.7 189.7 3.40 0.095 0.338
 21 d of lactation 174.1 175.2 177.6 177.8 5.67 0.611 0.940
 Lactation change (d 0 to 21) −5.5 −14.1 −9.1 −11.8 4.32 0.492 0.509
Backfat thickness (mm)
 At mating 20.8 21.5 19.7 20.5 1.48 0.694 0.965
 110 d of gestation 25.2 27.4 24.6 27.7 1.86 0.603 0.821
 Gestation gain (d 0 to 110) 4.4 5.9 4.9 7.2 1.31 0.243 0.786
 24 h postpartum 22.8 25.4 22.6 24.6 1.97 0.762 0.879
 21 d of lactation 19.2 20.9 19.9 22.2 1.72 0.333 0.881
 Lactation change (d 0 to 21) −3.6 −4.4 −2.7 −2.4 0.92 0.224 0.563
Lactation feed intake (kg/d) 3.75 4.11 4.17 4.08 0.457 0.626 0.626
Weaning to estrus interval (d) 5.2 5.1 5.3 5.0 0.42 0.836 0.746
1

Standard error of the mean.

Table 3

Effect of CP levels in gestation diets on litter size and litter performance of primiparous sows

Item Protein level in gestation (%) SEM1 p-value


11.44 12.93 15.04 17.13 Linear Quadratic
No. of sows 5 7 6 6
Litter size, no. of piglets
 Total born 12.20 11.86 12.00 10.50 0.806 0.199 0.482
 Stillbirth 0.40 0.29 0.67 0.00 0.259 0.502 0.300
 Mummified 0.00 0.00 0.00 0.00 - - -
 Born alive 11.80 11.57 11.33 10.50 0.838 0.299 0.722
 After cross-fostering 11.60 11.43 11.50 11.50 0.223 0.827 0.706
 Weaning pigs (d 21) 11.00 11.14 11.33 11.17 0.243 0.547 0.533
 Preweaning mortality (%) 5.00 2.38 1.52 2.90 1.723 0.381 0.260
Litter weight (kg)
 At birth 16.20 15.46 16.13 13.63 1.121 0.193 0.445
 After cross-fostering 14.58 14.91 15.52 15.22 0.764 0.486 0.683
 21 d of lactation 46.72 56.40 51.87 58.98 2.498 0.011 0.614
 Litter weight gain (d 0 to 21, kg/d) 1.54 1.96 1.72 2.10 0.108 0.008 0.874
Piglet weight (kg)
 At birth 1.29 1.33 1.35 1.33 0.067 0.651 0.656
 After cross-fostering 1.27 1.33 1.35 1.33 0.067 0.482 0.593
 21 d of lactation 4.25 5.06 4.60 5.31 0.257 0.032 0.844
 Piglet weight gain (d 0 to 21, kg/d) 0.14 0.18 0.16 0.19 0.011 0.035 0.952
1

Standard error of mean.

Table 4

Effect of CP levels in gestation diets on blood profiles of gilts in gestation1

Item Protein level in gestation (%) SEM2 p-value


11.44 12.93 15.04 17.13 Linear Quadratic
Plasma urea nitrogen (g/dL)3,4
 At mating5 10.9 10.9 10.9 10.9 - - -
 15 d 9.2 10.3 12.2 15.1 0.71 <0.001 0.225
 35 d 8.6 10.2 12.0 16.0 0.76 <0.001 0.130
 70 d 7.0 9.8 11.8 15.6 0.68 <0.001 0.447
 90 d 6.2 7.7 10.1 13.1 0.42 <0.001 0.113
 110 d 8.2 7.8 10.0 11.0 1.02 0.031 0.510
Plasma free fatty acids (μEq/L)3
 At mating 69.6 69.6 69.6 69.6 - - -
 15 d 33.4 42.4 45.8 29.0 4.10 0.600 0.006
 35 d 29.6 31.8 33.2 26.0 3.16 0.515 0.156
 70 d 29.4 34.4 36.8 27.4 3.56 0.824 0.061
 90 d 32.2 26.8 68.2 34.2 6.26 0.110 0.037
 110 d 108.0 127.4 132.6 85.5 6.06 0.356 0.794
Plasma glucose (mg/dL)3
 At mating 73.0 73.0 73.0 73.0 - - -
 15 d 61.0 68.4 68.2 63.2 2.92 0.631 0.050
 35 d 63.4 70.6 67.6 58.4 4.84 0.418 0.110
 70 d 70.2 64.4 54.2 65.6 4.19 0.218 0.057
 90 d 67.0 61.6 69.4 64.6 3.52 0.970 0.933
 110 d 78.4 77.6 73.2 76.4 6.06 0.706 0.746
1

Least squares means of 5 observations per treatment.

2

Standard error of mean.

3

Day effect (p<0.01; repeated measures ANOVA).

4

Day×treatment interaction (p<0.05; repeated measures ANOVA).

5

Blood samples (n = 11) were randomly taken from gilts immediately before mating.

Table 5

Effect of CP levels in gestation diets on blood profiles of primiparous sows and their progeny in lactation1

Item Protein level in gestation (%) SEM2 p-value


11.44 12.93 15.04 17.13 Linear Quadratic
Sows
 Plasma urea nitrogen (g/dL)3,5
  24 h postpartum 8.8 11.7 13.8 14.6 0.96 0.001 0.294
  21 d of lactation 15.8 15.8 15.9 14.4 0.97 0.095 0.783
 Plasma free fatty acids (μEq/L)
  24 h postpartum 333.5 187.6 127.0 229.6 60.21 0.254 0.068
  21 d of lactation 164.6 335.8 200.8 163.5 68.30 0.625 0.194
 Plasma glucose (mg/dL)3
  24 h postpartum 97.8 89.0 99.0 92.2 6.04 0.804 0.871
  21 d of lactation 83.6 87.6 85.0 79.2 2.78 0.222 0.097
Nursing pigs
 Plasma urea nitrogen (g/dL)3
  At birth 16.4 19.1 14.5 19.1 2.32 0.724 0.684
  21 d of lactation 10.2 7.9 7.6 9.7 1.65 0.833 0.206
 Plasma glucose (mg/dL)4
  At birth 97.6 98.0 92.0 96.0 13.13 0.856 0.893
  21 d of lactation 116.8 118.6 105.8 115.0 4.77 0.407 0.450
1

Least squares means of 5 observations per treatment.

2

Standard error of mean.

3

Day effect (p<0.01; repeated measures ANOVA).

4

Day effect (p<0.05; repeated measures ANOVA).

5

Day×treatment interaction (p<0.01; repeated measures ANOVA).

Table 6

Effect of CP levels in gestation diets on milk composition of primiparous sows1

Item Protein level in gestation (%) SEM2 p-value


11.44 12.93 15.04 17.13 Linear Quadratic
Colostrum at 24 h postpartum (%)
 Fat 8.78 6.99 7.15 7.32 0.869 0.104 0.138
 Protein 8.01 8.64 7.79 7.41 1.145 0.611 0.664
 Lactose 3.80 3.89 4.03 4.04 0.227 0.415 0.862
 Total solids 25.68 22.86 22.05 21.84 1.896 0.165 0.523
 Solids not fat 11.58 12.30 11.75 11.36 0.813 0.743 0.501
Milk at 21 d of lactation (%)
 Fat 6.77 6.97 6.76 6.69 0.400 0.808 0.744
 Protein 4.85 4.64 4.78 4.83 0.121 0.871 0.304
 Lactose 5.40 5.59 5.52 5.58 0.065 0.117 0.301
 Total solids 19.13 19.22 19.05 19.19 0.450 0.995 0.955
 Solids not fat 10.31 10.21 10.27 10.39 0.120 0.578 0.387
1

Least squares means of 5 observations per treatment.

2

Standard error of mean.

Table 7

Effect of CP levels in gestation diets on amino acid composition (g/100 g milk protein) in colostrum of primiparous sows1

Item Protein level in gestation (%) SEM2 p-value


11.44 12.93 15.04 17.13 Linear Quadratic
Essential amino acids
 Arg 4.94 4.91 4.85 4.70 0.080 0.057 0.461
 His 2.72 2.63 2.60 2.73 0.040 0.958 0.021
 Ile 3.68 3.49 3.51 3.70 0.071 0.778 0.023
 Leu 9.13 9.27 9.10 9.26 0.135 0.710 0.954
 Lys 7.24 7.09 7.12 7.37 0.108 0.428 0.093
 Met 2.15 1.90 2.03 1.95 0.078 0.239 0.284
 Phe 4.20 4.24 4.25 4.18 0.080 0.932 0.493
 Thr 5.20 5.41 5.48 5.19 0.172 0.941 0.177
 Val 6.72 6.77 6.67 6.69 0.193 0.846 0.945
Non-essential amino acids
 Ala 4.08 4.14 4.14 4.14 0.050 0.362 0.552
 Asp 8.27 8.09 8.12 8.15 0.121 0.582 0.412
 Cys 1.74 1.77 1.83 1.53 0.054 0.040 0.011
 Glu 17.67 17.41 17.38 18.19 0.482 0.503 0.289
 Gly 3.11 3.29 3.25 3.05 0.083 0.586 0.047
 Pro 8.93 9.10 8.89 9.13 0.143 0.569 0.840
 Ser 5.78 5.97 6.05 5.70 0.125 0.811 0.059
 Tyr 4.49 4.54 4.74 4.33 0.121 0.657 0.080
1

Least squares means of 5 observations per treatment.

2

Standard error of mean.

Table 8

Effect of CP levels in gestation diets on amino acid composition (g/100 g milk protein) in milk of primiparous sows at 21 d of lactation1

Item Protein level in gestation (%) SEM2 p-value


11.44 12.93 15.04 17.13 Linear Quadratic
Essential amino acids
 Arg 4.59 4.64 4.52 4.43 0.040 0.009 0.145
 His 2.67 2.72 2.69 2.67 0.038 0.944 0.379
 Ile 3.93 3.93 3.94 3.84 0.051 0.307 0.377
 Leu 8.56 8.36 8.51 8.61 0.097 0.492 0.153
 Lys 7.58 7.55 7.59 7.50 0.059 0.490 0.642
 Met 2.54 2.02 2.22 1.84 0.101 0.002 0.505
 Phe 3.84 3.78 3.80 3.84 0.038 0.847 0.188
 Thr 4.26 4.13 4.23 4.23 0.040 0.751 0.119
 Val 5.89 5.99 5.96 5.94 0.048 0.538 0.229
Non-essential amino acids
 Ala 3.51 3.53 3.56 3.52 0.055 0.811 0.697
 Asp 8.11 8.06 8.03 7.96 0.067 0.151 0.836
 Cys 1.56 1.46 1.50 1.24 0.071 0.019 0.297
 Glu 20.42 20.91 20.72 21.13 0.139 0.012 0.751
 Gly 2.96 3.08 2.98 3.07 0.067 0.491 0.837
 Pro 10.47 10.84 10.58 11.09 0.174 0.071 0.690
 Ser 5.15 5.04 5.19 5.15 0.041 0.419 0.393
 Tyr 3.98 3.98 3.99 3.90 0.081 0.575 0.637
1

Least squares means of 5 observations per treatment.

2

Standard error of mean.