4.5 Article

Processed soybean meal as an alternative protein source for yellow perch (Perca flavescens) feed

Journal

AQUACULTURE NUTRITION
Volume 25, Issue 4, Pages 917-931

Publisher

WILEY
DOI: 10.1111/anu.12911

Keywords

antinutritional factors; exogenous enzymes cocktail; growth; modified soybean meal; protein metabolism and antioxidant enzymes; yellow perch (Perca flavescens)

Categories

Funding

  1. Ohio Soybean Council, USA
  2. U.S. Department of Agriculture
  3. Ohio State University
  4. Ohio Agricultural Research and Development Center

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The goal of this study was to compare conventional soybean meal (SBM) with modified SBM (MSBM) after chemical and enzyme pretreatment to potentially reduce the antinutritional factors (ANF), as a fishmeal (FM) replacer at 50% or 100% in the diets of yellow perch (Perca flavescens). Half of the SBM and MSBM diets contained an enzyme cocktail (of phytase and carbohydrate-degrading enzyme), and the other half received no enzyme supplementations. Fingerlings (297; initial weight, 11.01 +/- 0.19 g) were randomly distributed over nine treatments, in triplicate, and fed these isonitrogenous diets (crude protein 410 g/kg) that included replacing FM with SBM at 50% or 100% without or with enzyme supplementations (S50, S100, S50+E or S100+E, respectively), MSMB at 50% or 100% without or with enzyme supplementations (MS50, MS100, MS50+E or MS100+E, respectively) or a control FM-based diet. After 10 weeks, the growth performance, feeding efficiencies, proximate composition, intestinal/pyloric caeca digestive enzymes and liver metabolic/antioxidant enzymes in P. flavescens were measured. The highest (p < 0.05) growth performance and nutrient utilization parameters (protein efficiency ratio and protein productive value, PPV) were observed for the MS50+E group, which was not statistically different to parameters for the control and MS50 groups, and significantly (p < 0.05) higher than all other groups. The lowest and highest growth performance and feed conversion ratios, respectively, were observed in the S100, S100+E and MS100 groups. The highest protease activity (in both intestine and pyloric caeca) was observed for the control group, but was significantly similar to MS50, MS50+E and S50+E groups. The lowest value was observed for 100% replacement of FM protein by SBM and MSBM fed groups. However, inclusion of exogenous enzymes in feed showed positive effects in MS50+E (compared to MS50) for PPV, lipid productive value and amylase activity in the intestine. Activity of protein metabolism enzymes (i.e., alanine transaminase and aspartate aminotransferase) in the liver was the highest in the control group, which was similar (p < 0.05) to the MS50+E and MS50 groups. Antioxidant enzymes (catalase, superoxide dismutase and glutathione peroxidase) in the liver were the lowest in the control group, which was significantly similar (p < 0.05) to the group given the feed with 50% replacement of FM protein. Complete (100%) replacement of FM protein exhibited the highest antioxidant enzyme activity. Conclusively, performance of the MS50 and MS50+E groups was similar to the FM group and better than SBM group; therefore, MSBM with high protein and low ANFs has considerable potential as an alternative to FM in aquafeed.

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