EFFECTS OF AUTOCLAVED YEAST CULTURES (SACCHAROMYCES CEREVISIAE) AND LIVE YEAST ON RUMINAL FERMENTATION IN VITRO

Document Type : Research article

Authors

1 Department of Nutrition and Clinical Nutrition, Faculty of Veterinary Medicine, Assiut University, Assiut, Egypt

2 Dept. of Animal Hygiene, South Valley University, Qena, Egypt.

3 Institute of Animal Nutrition, Dept. of Farm Animals and Veterinary Public Health, University of Veterinary Medicine, Vienna, Austria

Abstract

The objective of this study is to determine whether an autoclaved yeast culture of Saccharomyces cerevisiae or live yeast has an effect on the parameters of ruminal fermentation. For this purpose, autoclaved yeast cultures and live yeast were tested simultaneously by the rumen simulation technique (Rusitec). Each fermentation vessel received daily  15 g feed bag consists of 7.5 g dried basal feed (5 g grass silage + 2.5 g corn silage) and 7.5 g concentrate pellets. Two experiments with two fermentation vessels were carried out. In exp 1 the 1st vessel (control) received 7.5 g energy concentrate in addition to 7.5 g dried basal feed. The second fermentation vessel (T1) received 5 g energy concentrate plus 2.5 g protein concentrate containing autoclaved yeast culture in addition 7.5 g basal feed. In exp 2 the vessel 1 received the same control diet as in experiment one, while vessel 2 (T2) received 5 g energy concentrate + 2.5 g of protein concentrate containing autoclaved yeast culture and live yeast in addition to 7.5 g basal feed. Yeast culture influenced the ruminal fermentation kinetics in terms of lower (P<0.05) gas volume and higher acetate (mol %), with a concomitant decrease in iso-valerate (mol %) in experiment 1, moreover, yeast culture numerically not statistically increase individual and total volatile fatty acids. in experiment 2, the living yeast cells decreased gas volume more than yeast culture but not alter any other rumen fermentation kinetics. In conclusion autoclaved yeast culture and living yeast cells had beneficial effects on rumen fermentation and this effect was more pronounced with live yeast culture.

Keywords

Full Text

Dept. of Nutrition and Clinical Nutrition,

Faculty of Veterinary Medicine, AssiutUniversity, Assiut, Egypt.

E-mail:  abdelrheem@yahoo.com

 

Effects of autoclaved yeast cultures (Saccharomyces cerevisiae) and live yeast on ruminal fermentation in vitro

(With 7 Tables and One Figure)

 

By

Sh.M. Abdel-Raheem, Wageha A. Awad*,             C. Iben**and J. Böhm**

*Dept. of Animal Hygiene, SouthValleyUniversity, Qena, Egypt. 

 

**Institute of Animal Nutrition, Dept. of Farm Animals and Veterinary Public Health, University of Veterinary Medicine, Vienna, Austria

(Received at 26/11/2011)

 

أثر إضافة کل من مستنبت الخميرة المعقمة والخميرة الحية علي مقاييس التخمر في الکرش معمليا

 

شريف محمد عبد الرحيم ، وجيهة عوض ، کرستينا إيبن ، يوسف بم

 

أجريت هذه الدراسة لمعرفة أثر إضافة الخميرة المعقمة أو الحية علي مقاييس التخمر في  الکرش. لذلک تم إجراء تجربتين باستخدام جهاز محاکاة الکرش المکون من وعاءين للتخمر يحتوي کل منهما علي سائل الکرش. وُضع في کل وعاء کيس نايلون يحتوي علي 15 جرام من العليقة المکونة من 7.5 جرام من المادة المالئة (سيلاج الحشائش وسيلاج الذرة) وکذلک 7.5 جرام من المادة المرکزة هذا مع استبدال الأکياس کل 48 ساعة لمدة 10 أيام. في التجربة الأولي احتوي وعاء التخمر الأول علي العليقة الضابطة (الخالية من الخميرة بنوعيها) والمکونة من 7.5 جرام من مرکزات الطاقة بالإضافة إلي 7.5 جرام من المادة المالئة سالفة الذکر. في حين احتوي وعاء التخمر الثاني علي 5 جرام من مرکزات الطاقة وکذلک 2.5 جرام من مرکزات البروتين المزودة بالخميرة المعقمة بالإضافة إلي 7.5 جرام من المادة المالئة. هذا وقد اُستخدم الوعاء الأول کعليقه ضابطة في التجربة الثانية حيث احتوي علي 7.5 جرام من المادة المالئة و 7.5 جرام من مرکزات الطاقة في حين احتوي الوعاء الثاني علي 5 جرام من مرکزات الطاقة وکذلک 2.5 جرام من مرکزات البروتين المزودة بالخميرة المعقمة بالإضافة إلي الخميرة الحية بالاضافة الي 7.5 جرام من المادة المالئة. أظهرت النتائج أن إضافة مستنبت الخميرةأحدث تغييرات في مقاييس تخمر الکرش  علي هيئة زيادة معنوية في ترکيز حامض ألخليک مع زيادة رقمية في باقي الأحماض الطيارة الفردية وکذلک الترکيز الکلي للأحماض. وذلک بالتوازي مع نقص معنوي في حامض ايزوفاليرک وکذلک حجم الغاز الکلي الناتج من عملية التخمر, بينما أدت إضافة الخميرة الحية إلي نقص حجم الغاز الکلي ولم يکن لها أي اثر معنوي علي أي من مقاييس التخمر. مما سبق يتضح أن مستنبت الخميرةالمعقمةوکذلک الخميرة الحية توثر علي مقاييس الکرش وقد کان هذا التغيير أکثر وضوحا مع الخميرة الحية تحت ظروف التجربة الحالية.

 

SUMMARY

 

The objective of this study is to determine whether an autoclaved yeast culture of Saccharomyces cerevisiae or live yeast has an effect on the parameters of ruminal fermentation. For this purpose, autoclaved yeast cultures and live yeast were tested simultaneously by the rumen simulation technique (Rusitec). Each fermentation vessel received daily  15 g feed bag consists of 7.5 g dried basal feed (5 g grass silage + 2.5 g corn silage) and 7.5 g concentrate pellets. Two experiments with two fermentation vessels were carried out. In exp 1 the 1st vessel (control) received 7.5 g energy concentrate in addition to 7.5 g dried basal feed. The second fermentation vessel (T1) received 5 g energy concentrate plus 2.5 g protein concentrate containing autoclaved yeast culture in addition 7.5 g basal feed. In exp 2 the vessel 1 received the same control diet as in experiment one, while vessel 2 (T2) received 5 g energy concentrate + 2.5 g of protein concentrate containing autoclaved yeast culture and live yeast in addition to 7.5 g basal feed. Yeast culture influenced the ruminal fermentation kinetics in terms of lower (P<0.05) gas volume and higher acetate (mol %), with a concomitant decrease in iso-valerate (mol %) in experiment 1, moreover, yeast culture numerically not statistically increase individual and total volatile fatty acids. in experiment 2, the living yeast cells decreased gas volume more than yeast culture but not alter any other rumen fermentation kinetics. In conclusion autoclaved yeast culture and living yeast cells had beneficial effects on rumen fermentation and this effect was more pronounced with live yeast culture.

 

Key words: Autoclaved yeast culture, live yeast, Rusitec,

fermentation parameters

 

 

 

 

Introduction

 

Addition of Saccharomyces cerevisiae cultures to ruminant diets improved the digestibility of dry matter, crude protein, and hemicellulose; increased ruminal bacterial numbers; decreased ruminal lactate concentrations; and increased milk production of cows in early lactation (Gomez-Alarcon et al., 1990). Saccharomyces cerevisiae cultures provide soluble growth factors (i.e., organic acids, B vitamins, and amino acids) that are required by ruminal bacteria for growth on lactate (Nisbet and Martin, 1991). Dietary supplements of yeast culture, based on dried Saccharomyces cerevisiae, have been reported to increase productivity in ruminants, by a mechanism that results in an increased viable count of bacteria in the rumen which may lead to improved protein flow to the small intestine (Newbold 1995). Nisbet and Martin (1991) reported that S. cerevisiae stimulated the growth of the prominent lactic acid-utilizing rumen bacterium, Selenomonas ruminantium, in pure culture, apparently because dicarboxylic acids in the yeast stimulated lactate uptake by the bacterium. Moreover, Newbold et al. (1996) suggested two modes of action of yeast in stimulating rumen fermentation; the first, yeast respiratory activity protects anaerobic rumen bacteria from damage by oxgen, the second, yeast provides malic and other dicarboxylic acids which stimulate the growth of some rumen bacteria. They concluded that the stimulation of rumen bacteria by        S. cerevisiaeis at least partly dependent on its respiratory activity, and isnot mediated by malic acid. Ruminal digestion of low quality feedstuffs provides the host volatile fatty acids and microbial protein to support energy requirements for sustenance, growth and work. Only about 10– 35% of dietary energy consumed by the ruminant is conserved, however, improvements in digestive efficiency could improve ruminant animal production, with lowering input costs and undesired environmental impacts (Varga and Kolver, 1997). Ruminal methane production, for instance, results in the inefficient conversion of potentially energy-yielding substrates into a form that can not be conserved by the host. There have been many attempts to manipulate the rumen fermentation with the intention of increasing the production of propionate and reducing the production of methane. There are advantages in both directions, since the production of methane represents a direct loss of energy, while propionic acid is an important precursor for gluconeogenesis.

 

 

The rumen simulation technique (Rusitec) makes it possible to examine the direct effects of autoclaved yeast cultures or live yeast as additives in ruminant diets independent of the host ruminant. Therefore, the objective of this study was to investigate the effect of two types of yeast (autoclaved or live) on rumen fermentation parameters in vitro.

 

Materialsand methods

 

The experimental design is illustrated in Table 1. Two experiments were carried out using two Rusitec fermentation vessels described by Czerkawski and Breckenridge (1977). The incubation vessels was filled with rumen fluid. Rumen contents were taken from a rumen of fistulated cow that was maintained on a diet of grass hay and grain concentrates. Animals had free access to hay, water, and a vitamin-enriched salt lick. Each vessel was loaded with 2 nylon bags. The nylon bags (70×120 mm) had a pore size of 150 μm which is usually used for in vitro rumen fermentation studies (Öztürk, 2003). At the start of the trial, one bag was filled with 80 g of solid rumen contents to inoculate particle-associated microorganisms into the system and the other with the daily tested diets. The nylon bag with solid rumen contents was replaced after 24 h of incubation with a bag containing the diet. The feed bag was changed after 48 h so that 2 bags were always present. This gave a retention time of 48 h for feed. Bags were exchanged under anaerobic conditions using N2 to flush the incubation vessels. To maintain conditions as close to those of the in vivo rumen as possible, the incubation temperature was 39°C and rumen fluid turnover was simulated by modified artificial saliva. By moving the inner vessel up and down continuously rumen motility was simulated and exchange between the fluid and particle phases was completely done. In both experiments each vessel received 7.5 g dried basal feed (5 g grass silage + 2.5 g corn silage) and 7.5 g concentrate. In exp 1 the 1st vessel (control) received 7.5 g of energy concentrate (kombilac 16) beside 7.5 g of the basal feed, while the second fermentation vessel (T1) received a concentrate mixture consisting of 5 g energy concentrate (Kombilac 16) and 2.5 g protein concentrate containing 2.47% autoclaved yeast culture (Rumenac Prolactin) in addition to 7.5 g basal feed. In Exp. 2 vessel 1 received the same control diet as in experiment 1, however, vessel 2 received 5 g of energy concentrate plus 2.5 g protein concentrate containing autoclaved yeast (Rumenac Prolactin) in addition to a feed additives containing live yeast (RumexSC) beside the basal feed. The chemical composition of the experimental diets is presented in Table 2. An equilibration period of 5 days was allowed before the rumen fluid and the effluent samples were collected for the next 5 days (collection period) and repeated 3 times, and sequential samples of ruminal fluid were taken from inside the vessels before replacing the feed bags. Gas volume was determined daily by gas bag. The liquid flow through the vessels was maintained by continuous infusion of a buffer solution (pH 7.4) at the rate of 750 ml/day the composition of the buffer is shown in Table 3 according to McDougall’s (1948). All additives were supported by Fixkraft® company (Enns, Austria) except RumexSC was supported by Delacon company®, Austria.

 

Analytical procedures and samplings

Most of the analytical procedures used were as described by Czerkawski and Breckenridge (1977). The pH and redox potential values were measured daily in each vessel at the time of feeding using a pH and redox electrodes (Typ 408, Mettler Toledo, Steinbach, Germany) connected to a Knick pH meter (digital pH meter 646, Knick, Berlin, Germany). Liquid effluent was collected daily and samples were taken for analyses of microbial particulate DM. Rumen fluid samples was mixed with oxalic acid (0.1 mol/l), sodium azide (40 mmol/l) and capronic acid (0.1 mmol/l) as internal standard, centrifuged and the supernatant was analyzed for short chain fatty acids (SCFAs) by gas chromatography (Agilent 6890 N GC) equipped with a 30 m x 530µm x 0.1µm capillary column with flame ionization detector according to the method described by Schafer, (1995). Rumen ammonia was analysed using test kits (Sigma – Aldrich) by spectrophotometer (Hitachi, U- 3000, USA)

 

Statistical analyses

Statistical analyses were conducted with the Statistical Package for Social Science (SPSS for Windows Version 13; SPSS GmbH, Munich, Germany) to determine if the variables differed between groups. Differences between the means were compared by independent t-test. Probability values of P<0.05 were considered as significant. Values in tables are means ± SD.

 

 

 

 

Results

 

Effects of yeast culture on ruminal fermentation in vitro are shown in Tables 4, 5, 6 and 7. In experiment 1: the addition of autoclaved yeast culture in the fermentation vessel significantly decreased the gas volume and the molar proportion of isovalerate volatile fatty acid in concomitant with significant increase in the molar proportion of ruminal acetate. In addition, there are numerical increases in the effluent microbial dry matter out put (particulate dry matter, PDM), the concentration of propionate, other individuals and the total daily volatile fatty acids (VFA) by the addition of autoclaved yeast culture to the fermentation vessels. The autoclaved yeast culture exhibit no significant (P > 0.05) impact on rumen pH, redox potential and ammonia concentration in experiment 1.

In experiment 2: asignificant reduction in gas volume from vessel 2 receiving the living yeast cell in comparison with vessel receiving the control diet. In addition, there are numerical increases in the individual and total volatile fatty acids. No significant impact was noticed in experiment 2 on other rumen fermentation kinetics.

 

Table 1: Experimental design. 

 

Experiment

Vessel 1

Vessel 2

1

7.5 g basal feed* (roughages)

7.5 Energy Concentrate (kombilac 16)

  (control)

 

7.5 g basal feed (roughages)

5 g Energy Concentrates

2.5 g protein concentrate containing autoclaved yeast culture (Ruminac prolactin (T1)

2

7.5 g basal feed (roughages)

7.5 Energy Concentrate(kombilac 16)

  (control)

 

7.5 g basal feed (roughages)

5 g Energy Concentrates

2.5 g protein concentrate containing autoclaved yeast culture (Ruminac prolactin + live yeast (RumexSC) (T2)

 

* Basal feed = 5 g grass silage + 2.5 g corn silage

 Ruminac prolactin contains autoclaved yeast culture (2.47 %)

 

 

Table 2: Chemical composition of the experimental diet (%, as fed basis)

 

Item

DM

OM

CP

EE

CF

    NFE

Ash

GE1

Grass silage

53.1

47.3

9.5

1

11.9

24.9

5.8

10.138

Corn silage

35.4

34.1

2.3

1.5

6.6

23.7

1.3

6.656

Kombilac 16

87.6

82.7

16.9

3

5.3

57.5

4.9

14.857

Rumenac prolactin

90

85

20.3

2.8

5.2

56.7

5

15.369

Rumenac prolactin + RumexSC

87.4

82.3

20.4

3.1

4.8

54

5.1

14.506

 

 

1 GE KJ/g = Determined by bomb calorimeter

Kombilac 16= Energy concentrate contains 16 % CP and 7 MJ NEL, Rumenac prolactin= protein concentrate contains 20 % CP, 7.5 MJ NEL and yeast culture (2.47 %), RumexSC= (natural feed additives) containing live yeast.

 

Table 3: Chemical composition of modified artificial saliva (RUSITEC buffer)

 

Ingredient

g/l

mmol/l

 

Sodium chloride (NaCl)

 

1.6380

 

28

Potassium chloride (KCl)

0.573

7.69

Calcium chloride (CaCl2 2H2O)

0.0323

0.22

Magnesium chloride (Mg Cl2 6 H2O)

0.128

0.63

Ammonium chloride (NH4 Cl)

0.267

5.00

Disodium hydrogen phosphate (Na2HPO4 12 H2O)

3.58

10.00

Sodium Hydrogen phosphate (NaH2PO4  H2O)

1.38

10.00

Sodium bicarbonate (NaHCO3 )

 

8.224

97.90

 


Table 4: Effect of autoclaved yeast culture on rumen fermentation parameters in Rusitec (Exp.1)

 

Items

Control

Autoclaved yeast culture

P

Ph

6.47 ± 0.08

6.45 ± 0.04

0.2

Redox potential (mv)

-286.5 ± 19

-281± 21

1.2

Gas volume (ml)

1263 ± 84a

1150 ± 77b

0.000

Ammonia (g/l)

0.20 ± 0.05

0.19 ± 0.06

0.8

Effluent PDM (g/l)

0.50 ± 0.06

0.71± 0.14

0.15

 

a, b Means within a row with different superscripts are significantly different (P <005).

PDM = particulate dry matter (microbial output)

 

Table 5: Effect of autoclaved yeast culture on rumen VFA and the molar % VFA (Exp. 1)

 

Acids

Control

Autoclaved yeast culture

P

Acetate (mmol/l)

19.4 ± 2.1

20.9± 4.6

0.18

Propionate (mmol/l)

7.8 ± 0.6

8.1 ±1.7

0.4

i-butyrate (mmol/l)

0.27 ± 0.03

0.3 ± 0.1

0.25

n-butyrate (mmol/l)

6.10 ± 0.6

6.4 ± 1.3

0.18

i-valerate (mmol/l)

1.7 ± 0.3

1.5 ± 0.3

0.08

n-valerate (mmol/l)

2.0 ± 0.4

2.1 ± 0.6

0.62

Total VFA (mmol/l)

37.1 ± 3.9

39.2 ± 8.4

0.18

………………mol %.....................

Acetate

52.0 ± 0.3 a

53.2 ± 0.5 b

0.001

Propionate

20.9 ± 0.9

20.7 ± 0.4

0.25

n-butyrate

16.4 ± 0.5

16.4 ± 0.2

0.15

i-butyrate

0.7 ± 0.1

0.7 ± 0.1

0.08

i-valerate

4.4 ± 0.5 a

3.7 ± 0.4 b

0.62

n-valerate

5.4 ± 0.5

5.3 ± 0.4

0.3
         

 

 

 

Table 6: Effect of live yeast on fermentation parameters (Exp. 2)

 

Items

Control

Live yeast

P

pH

6.51 ± 0.05

6.49 ± 0.08

0.3

Redox potential (mv)

-295.7 ± 25

-288.2 ± 16

0.08

Gas volume (ml)

1305 ± 52 a

1080 ± 81b

0.02

Ammonia (g/l)

0.23 ± 0.03

0.17 ± 0.03

0.09

Effluent PDM (g/l)

0.51± 0.09

0.63 ± 0.09

0.08

 

 

a, b Means within a row with different superscripts are significantly different (P <005).

PDM = particulate dry matter (microbial output)

 

Table 7: Effect of live yeast on rumen VFA and the molar % VFA   (Exp. 2)

 

Acids

 Control

Live yeast

P

Acetate (mmol/l)

19.1 ± 5.1

20.0 ± 3.1

0.4

Propionate (mmol/l)

8.8 ± 2.6

9.2 ± 1.6

0.51

i-butyrate (mmol/l)

0.3 ± 0.1

0.3 ± 0.1

0.09

n-butyrate (mmol/l)

5.5 ± 1.6

6.2 ± 0.9

0.54

i-valerate (mmol/l)

1.5 ± 0.6

1.73 ± 0.6

0.35

n-valerate (mmol/l)

2.3 ± 0.8

2.5 ± .5

0.22

Total VFA (mmol/l)

37.5 ± 10.7

40 ± 6.7

0.08

………………mol %.....................

Acetate

51.3 ± 1.39

50.1 ± 1.0

0.43

Propionate

23.4 ± 0.8

22.9 ± 0.6

0.2

n-butyrate

14.7 ± 0.9

15.6 ± 0.5

0.09

i-butyrate

0.8 ± 0.1

0.8 ± 0.01

0.67

i-valerate

3.8 ± 0.6

4.2 ± 0.8

0.32

n-valerate

6.0 ± 0.4

6.3 ± 0.5

0.24

 

 

 
 

B
 

 

 

 

 
 
 
 

 

 

 

 

 

 

 

 
 
 
 

 

 

 

 

 

 

 

 

 

 

 

 

 

 

 

Fig. 1: A and B (Rusitec) Rumen Simulation technique design used in the experiment. C. Schematic diagram of one vessel of rusitec adapted from Czerkawski and Breckenridge (1977).

Discussion

 

In animals fed high-energy diets, decreased lactic acid concentrations are associated with higher ruminal pH, and are characteristic of much more stable ruminal fermentation. These alterations in ruminal fermentations can be expected for improved digestion, and could also be reflected in improved intake. The ability of yeast to prevent the accumulation of lactic acid in the rumen suggests a role for viable yeast in overcoming ruminal dysfunctions associated with the use of high energy diets used in both high-producing dairy and fast-growing beef cattle. The significant increase in acetate and numerical increase in some individual and total VFA by the addition of yeast culture was in agreement with results of Callaway and Martin, (1997) and Oeztuerk, (2009). They reported that yeast culture increased the concentrations of acetate and total volatile fatty acids that produced by Sel. ruminantium HD4 and increased the concentrations of propionate and total volatile fatty acids that produced by Sel. ruminantium H18.  Callaway and Martin, (1997) suggested that, yeast culture provides soluble growth factors (i.e., organic acids, B vitamins, and amino acids) which stimulate growth of ruminal bacteria that utilize lactate and digest cellulose. So, dietary supplementation with yeast cultures that are high in these growth factors may improve ruminal fermentation. Moreover, Wallace and Newbold (1992) concluded that the production benefits seen when yeast culture is added to the diet arise from changes in the stoichiometry of VFA formation. The increase in the proportion of acetate was also observed by the experiment of Mutsvangwa et al. (1992) with yeast culture. The positive effect of living yeast cell in experiment 2 was in agreement with that of Dawson et al. (1990) and Callaway and Martin, (1997) who reported that heat inactivated yeast culture preparations have no effect on ruminal bacterial growth, suggesting that live yeast cells are necessary for the stimulation of growth of lactate utilizing bacteria Sel. ruminantium.

The decrease in gas production which is mainly methane is a promising result, because methane emissions represent losses of up to 15% of gross energy intake for forage-fed cattle and losses of 2–4% for cattle consuming diets rich in readily fermentable substates (Johnson and Johnson, 1995). There have been many attempts to manipulate the rumen fermentation with the intention of increasing the production of propionate and reducing the production of methane. There are advantages in both directions, since the production of methane represents a direct loss of energy while, propionic acid is an important precursor for gluconeogenesis. It can thus have a protein sparing role since amino acids are the other main source of glucose precursors (Leng, 1970).

In the current study, many of the changes associated with the addition of yeast cultures were marginal and often not statistically significant. This makes interpretation difficult, In conclusion, these results indicated that, the addition of either autoclaved or live yeast cultures stimulated ruminal fermentation and this effect was more pronounced with live yeast culture.

 

References

 

Callaway, E.S. and Martin, S.A. (1997): Effects of a Saccharomyces cerevisiae culture on ruminal bacteria that utilize lactate and digest cellulose. Journal of Dairy Science, 80: No. 9.

Czerkawski J.W. and Breckenridge, G. (1977): Design and development of a long-term rumen simulation technique (Rusitec). Brit. J. Nutr. 38: 371-384.

Dawson, K.A.; Newman, K.E. and Boling, J.A. (1990): Effects of microbial supplements containing yeast and lactobacilli on roughage-fed ruminal microbial cativities. J. Anim. Sci. 68: 3392.

Gomez-Alarcon, R.A.; Dudas, C. and Huber, J.T. (1990): Influence of cultures of Aspergillus oryzae on rumen and total tract digestibility of dietary components. J. Dairy Sci. 73: 703.

Johnson, K.A. and Johnson, D.E. (1995): Methane emissions from cattle. J. Anim. Sci. 73: 2483–2492.

Leng, R.A. (1970): Glucose synthesis in ruminants. Adv. in Vet. Sci., 14: 209.

McDougall, E.I. (1948): Studies on ruminant saliva. 1. the composition and out put of sheep`s Saliva. Biochemical journal, 43, (1), 99.

Mutsvangwa, T.; Edwards, I.E.; Topps, J.H. and Peterson, G.F.M. (1992): The effect of dietary inclusion of yeast culture (Yea-Sacc) on patterns of rumen fermentation, food intake and growth of intensively fed bulls. Anim. Prod. 55: 35-40.

Newbold, C. J.; Wallace, R.J.; Chen, X.B. and McIntosh, F. (1995): Different strains of Saccharomyces cerevisiae differ in their effects on rumen fermentation both in vitro and in sheep. J. Anim. Sci. 73: 1811–1818.

Newbold, C.J.; Wallace, R.J. and McIntosh, F. (1996): Mode of action of the yeast Sacchavomyces cerevisiae as a feed additive for ruminants.British Journal of' Nutrition (1996), 76, 249-261

Nisbet, D.J. and Martin, S.A. (1991): The effect of Saccharomyces cerevisiae culture on lactate utilization by the ruminal bacterium Selenomonas ruminantium. J. Anim. Sci. 69:     4628–4633.

Öztürk, H. (2003): In-vitro-Studien zum Einfl uss von Topinamburmehl und Saccharomyces boulardii auf den mikrobiellen Vormagenstoffwechsel. Dissertation, Tierärztliche Hochschule, Hannover(Germany), pp. 88.

Oeztuerk, H. (2009): Effects of live and autoclaved yeast cultures on ruminal fermentation in vitro. Journal of Animal and Feed Sciences, 18: 142–150.

Schäfer, K. (1995): Analysis of short chain fatty acids from different intestinal samples by capillary gas chromatography. Chromatographia, 40: 550-556.

Varga, G.A. and Kolver, E.S. (1997): Microbial and animal limitations to fiber digestion and utilization. J. Nutr. 127: 819S–823S.

Wallace, R.J. and Newbold, C.J. (1992): Probiotics for Ruminants. In: R. Fuller (Ed.) Probiotics: The Scientific Basis. p 317. Chapman and Hall, London.

 

 

 

 

 

 

 

 

 

 

 

 

 

 

 

 

 

References

References
 
Callaway, E.S. and Martin, S.A. (1997): Effects of a Saccharomyces cerevisiae culture on ruminal bacteria that utilize lactate and digest cellulose. Journal of Dairy Science, 80: No. 9.
Czerkawski J.W. and Breckenridge, G. (1977): Design and development of a long-term rumen simulation technique (Rusitec). Brit. J. Nutr. 38: 371-384.
Dawson, K.A.; Newman, K.E. and Boling, J.A. (1990): Effects of microbial supplements containing yeast and lactobacilli on roughage-fed ruminal microbial cativities. J. Anim. Sci. 68: 3392.
Gomez-Alarcon, R.A.; Dudas, C. and Huber, J.T. (1990): Influence of cultures of Aspergillus oryzae on rumen and total tract digestibility of dietary components. J. Dairy Sci. 73: 703.
Johnson, K.A. and Johnson, D.E. (1995): Methane emissions from cattle. J. Anim. Sci. 73: 2483–2492.
Leng, R.A. (1970): Glucose synthesis in ruminants. Adv. in Vet. Sci., 14: 209.
McDougall, E.I. (1948): Studies on ruminant saliva. 1. the composition and out put of sheep`s Saliva. Biochemical journal, 43, (1), 99.
Mutsvangwa, T.; Edwards, I.E.; Topps, J.H. and Peterson, G.F.M. (1992): The effect of dietary inclusion of yeast culture (Yea-Sacc) on patterns of rumen fermentation, food intake and growth of intensively fed bulls. Anim. Prod. 55: 35-40.
Newbold, C. J.; Wallace, R.J.; Chen, X.B. and McIntosh, F. (1995): Different strains of Saccharomyces cerevisiae differ in their effects on rumen fermentation both in vitro and in sheep. J. Anim. Sci. 73: 1811–1818.
Newbold, C.J.; Wallace, R.J. and McIntosh, F. (1996): Mode of action of the yeast Sacchavomyces cerevisiae as a feed additive for ruminants.British Journal of' Nutrition (1996), 76, 249-261
Nisbet, D.J. and Martin, S.A. (1991): The effect of Saccharomyces cerevisiae culture on lactate utilization by the ruminal bacterium Selenomonas ruminantium. J. Anim. Sci. 69:     4628–4633.
Öztürk, H. (2003): In-vitro-Studien zum Einfl uss von Topinamburmehl und Saccharomyces boulardii auf den mikrobiellen Vormagenstoffwechsel. Dissertation, Tierärztliche Hochschule, Hannover(Germany), pp. 88.
Oeztuerk, H. (2009): Effects of live and autoclaved yeast cultures on ruminal fermentation in vitro. Journal of Animal and Feed Sciences, 18: 142–150.
Schäfer, K. (1995): Analysis of short chain fatty acids from different intestinal samples by capillary gas chromatography. Chromatographia, 40: 550-556.
Varga, G.A. and Kolver, E.S. (1997): Microbial and animal limitations to fiber digestion and utilization. J. Nutr. 127: 819S–823S.
Wallace, R.J. and Newbold, C.J. (1992): Probiotics for Ruminants. In: R. Fuller (Ed.) Probiotics: The Scientific Basis. p 317. Chapman and Hall, London.

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