| Livestock Research for Rural Development 23 (11) 2011 | Guide for preparation of papers | LRRD Newsletter | Citation of this paper |
In order to facilitate fish cultivation in rural areas of the Neotropics, the potential of locally available aquatic macrophytes from northern Colombia (Lemna minor, Spirodela polyrhiza, Azolla filiculoides and Eichhornia crassipes) as alternative fish feedwas studied. Considering the importance of fermentation in the improvement of nutritional value of non-conventional feeds, the fermentation properties (Trial I)andthe effects of anaerobic fermentation on the nutritional quality of the selected aquatic plants (Trial II) were evaluated.
Results of the first trial indicated that although the fermentability coefficients (FC) of the selected aquatic macrophytes revealed a hardly fermentable material (FC< 35), the use of bacteria inoculants (Lactobacillus plantarum) and molasses (150 g/kg) resulted in a good silage quality. Results of the second trials howed that lactic acid fermentation positively affected the nutritional quality of the plants; since the concentration of some antinutritional substances and crude fibre content were reduced (P > 0.05).Fermentation of the tested aquatic macrophytes is highly recommendable to use them as fish feed supplement.
Key words: alternative fish feed, antinutritional factors, heavy metals, processing methods
In view of the increasing prices of ingredients for aquafeeds, the search for cheap and nutritionally balanced ingredients for fish feed has become an urgent need for the aquaculture sector. Particularly, the evaluation of the nutritional value and potential of locally available nutrient sources is an important aspect for the substitution of conventional fish feed ingredients.Aquatic macrophytes are among the most common plant materials in the tropical floodplain systems. They contribute to more than 60 % of the primary production in the Amazon floodplain (Leite et al 2002). In the Orinoco, they are also reported to be highly productive and to increase rapidly during high water (Vásquez 1989). In other freshwater ecosystems, they grow rapidly and remain during the whole year.
Due to their abundance, they contribute to eutrophication of water bodies (Xieet al 2004). Therefore, many researchers are looking for methods to control them effectively and others to convert them into utilizable resources (NAS 1976; Brabben 1993; Rodriguez and Preston 1996; Franklin et al 2008), both in industrial processes and at farm level (Leng 1999; Xiao et al 2009; Dordio et al 2010). In sustainable production systems, they have been frequently described as suitable alternative animal feed (Pípalová 2003; Sétliková and Adámek 2004; El-Sayed 2003; Bairagi et al 2002; Yılmaz et al 2004; Kalita et al 2007). However, their potential as fish feed should be evaluated on a local basis because of their variable composition, which is highly depending on the water quality conditions where the plants grow (Boyd 1971).
As other plant materials, aquatic macrophytes contain antinutritional substances that restrict their use as feed. To improve their nutritional value for fish and subsequently to increase their incorporation level into fish diets, they are commonly fermented.For instants, El-Sayed (2003) reported that fermentation is necessary when water hyacinth (Eichhornia crassipes) is included at levels of 20% or more into Nile tilapia diets. Likewise, Bairagi et al (2002) reported in their study that fermented Lemna leaf meal was better utilized than raw Lemna leaf meal in diets for rohu (Labeo rohita).
Although aquatic macrophytes are commonly found within the tropics, theyhave been poorly investigated as alternative or supplemented feed for the majority of native fish in Colombia. This may be due to the lack of information on their nutritional characteristics, fermentation properties and processing. Since this information is essential to increase their potential as fish feed, two separated trials were conducted to evaluate the fermentation properties (Trial I) and the effect of anaerobic fermentation on the nutritional quality and the content of antinutritional substances (Trial II) of Lemna minor, Spirodela polyrhiza, Azolla filiculoides and Eichhornia crassipes.
The aquatic macrophytes Spirodela polyrhiza (Giant Duckweed), Azolla sp. (fern Azolla) and Eichornia crassipes (Water Hyacinth) used in trial I were obtained from a commercial distributor (Wakus GmbH Berlin, Germany). Lemna minor (Duckweed) was obtained from the Botanical Garden of Berlin. The plant material was washed, oven dried and stored in plastic bags for preliminary analysis in laboratory. Eichhornia crassipes was previously separated into leaves and roots and chopped into small parts.
For fermentation, freshly harvested plants were mixed with a part of the oven dried aquatic macrophytes of the same sample to complete 350 to 450 g/kg dry matter. A total of 8 mixtures (two replicates per plant species) were used for lactic acid fermentation by addition of the commercial silage inoculants and of molasses at 150 g/kg as water soluble carbohydrates (WSC) source. Afterwards, the mixtures were vacuum packed into gas tight plastic bags according to the method described by Johnson et al (2005). Silages were maintained in an incubator for 60 days at 25°C.
For lactic acid fermentation, the commercial silage inoculants BIO-SIL® based on the lactic acid bacteria (LAB) strain Lactobacillus plantarum DSM 8862 and DSM 8866 (Dr. Pieper Technologie-und Produktentwicklung GmbH, Germany) was used. The inoculant solution was prepared according to the manufacturer’s information and used on a fixed dose of 2 ml/kg of plant material for a final inoculation rate of 3 x 105cfu/g.
The raw plant material was preliminarily analyzed in triplicate to determine the buffering capacity (BC) by electrometric titration (Automatic TitratorTyp AT 3 equipped with a glass electrode), nitrate content by potentiometric (ion selective electrode) and WSC content by anthrone method (Lengerken and Zimmermann 1991). The ratio WSC/BC was used to estimate the fermentability coefficients (FC).
Silages were also analyzed in triplicate. Acid concentration was determined by high-performance liquid chromatography (HPLC) according to Weiß and Kaiser (1995). Alcohols were determined chromatographically (GC). Ammonia was determined by Conway method according to Lengerken and Zimmermann (1991). The evaluation of the fermentation quality of silages was done on the basis of a chemical investigation according to the DLG (Deutsche Landwirtschafts-Gesellschaft) guidelines for silage quality proposed by Weißbach and Honig (1992).
The fermentability coefficient (FC) was used to judge the ensiling potential and was calculated according to the parameters on the silage fermentation:
- FC=DM (%) + 8 WSC/BC (Schmidt et al 1971).
The minimum dry matter content (DMmin) was calculated following the equation proposed by Kaiser et al (2002) as a function of nitrate content. As the DMmin content considered acceptable for ensiling in farm scale is 200 g/kg, whereas a DM content of 450 g/kgis considered as inhibitory limit value for clostridia growth in anaerobic conditions (McDonald et al 1991), samples were set to be ranged from 350 to 450 g/kgDM content.
The aquatic macrophytes Lemna minor (Duckweed), Spirodelapolyrhiza (Giant Duckweed), Azolla filiculoides (fern Azolla) and Eichhornia crassipes (Water Hyacinth) used in trial II were harvested as wild or uncultivated material from water bodies in northern Colombia. After collection and taxonomical identification, raw plant material was treated according to the procedures described above. A total of 12 mixtures, three replications per plant species, were prepared for fermentation. A sample of each mixture was taken before the vacuum packing to be analyzed for proximate composition. After 60 days of fermentation, samples were opened and analyzed again. Proximate analysis of the unfermented and fermented aquatic plants was performed following the AOAC (2005) procedures.
Samples of unfermented plant material were sent to a private laboratory to test the mineral and heavy metal content. Determination were done by atomic absorption spectrophotometry according to the AOAC methods 985.35 and 983.27 (AOAC 1995) and to the AOAC methods 995.11 and 999.11 (AOAC 2005). For amino acid composition samples of the unfermented material were also sent to the Nutrition and Food Research Center in Freising (Germany), where the determinations were done according to the methods of the European Commission due to regulation 159/2009. Amino acids were separated by ion chromatography and photometrically determined after Ninhydrin reaction by an amino acid analyzer (Biochrom 30).
Samples of unfermented and fermented plant material were also sent toa specialized laboratory for the determination of antinutritional substances. Trypsin inhibitory activity was determined by the enzymatic-colorimetric method using benzoyl-DL-arginine-p-nitroanilide (BAPA) as a substrate (Kakade et al 1969; Smith et al 1980). Hydrolysable and condensed tannins were determined by the spectrophotometric method using the Folin-Denis reagent (Price and Butler 1977) and vanillin hydrochloric acid (V-HCl) (Earp et al 1981), respectively. Phytates (as phytic acid activity) were determined by the enzymatic-spectrophotometric method at 492 nm (Cat No. K-PHYT, Megazyme International Ireland Ltd., Wicklow, Ireland). Oxalates were determined by HPLC.
To assess the separate and combined effect of the plant material (four species) and treatment (unfermented and fermented) on the nutritional composition (ash, protein and fibre content) of aquatic macrophytes a 4 x 2 factorial analysis of variance (ANOVA) was conducted. The means and standard error of means (SEM) for ash, protein and fibre content as a function of the two factors are presented in Table 5. The F test and Tukey's test for Post Hoc comparisons (P<0.05) were applied. All statistical analyses were performed using the SPSS (version 19) software package.
Table 1 shows the characteristics of the raw and lactic acid fermented aquatic macrophytes. Results indicated that dry matter content and water soluble carbohydrates (WSC) of all tested plants were very low, whereas crude fibre and ash content were relatively high. In addition, Spirodela and Lemna presented a high buffering capacity (BC). Thus, the fermentability coefficients of the raw aquatic macrophytes revealed a heavily fermentable material (FC<35).
The dry matter of the silages ranged within desirable values (395 - 446 g/kg). The pH values ranged from 3.92 to 4.26 indicating good silage quality. Ammonia-N content was low and ranged from 5 to 58 g/kg in CP, except for the stems of Eichhornia which reached a content of 164 g/kg ammonia-N in CP. Acetic acid content was also low in all samples. Silages were practically butyric and propionic acid-free. In contrast, concentrations of lactic acid were high and ranged from 74.2 (stems of Eichhornia) to 86.8 g/kg (leaves of Eichhornia). The evaluation of silage quality by DLG points for the tested silages obtained the highest mark.
Table 2 shows the chemical composition of the tested aquatic macrophytes grown in rural zones of Colombia. The crude protein content ranged between 157 and 212 g/kg DM, except for stems of Eichhornia with the lowest content (97.8 g/kg). Aquatic macrophytes have a relatively high crude fibre and ash content, and a low content of crude lipids. However, they are rich in minerals. Heavy metal concentrations of arsenic, selenium and mercury were not detectable. Cadmium and lead were detectable in low concentrations.
Table 3 shows the concentration of antinutritional substances in the raw and fermented aquatic macrophytes. Trypsin inhibitor, phytates (as phytic acid activity), soluble tannins and oxalates were detectable in all the raw aquatic plants, although the amounts did not exceed the tolerable limits for fish. Condensed tannins were not detectable in raw Lemna and Azolla, but were present in raw Spirodela and Eichhornia leaves. Trypsin inhibitor and oxalates were significantly reduced by the fermentation process, as well as phytates, except for Azolla, whose content of phytates did not change. Soluble and condensed tannins were not detectable in the fermented aquatic macrophytes.
|
Table 1. Chemical characteristics of raw and fermented aquatic macrophytes used in Trial I (expressed on dry matter basis except for DM which is on fresh basis). |
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|
Quality indicator |
Lemna minor |
Spirodela polyrhiza |
Azolla sp. |
E. crassipes |
E.crassipes |
|
(leaves) |
(stems) |
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|
Factors affecting fermentation |
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|
DM (g/kg), fresh |
56.4 |
55.4 |
50.2 |
95.8 |
52.1 |
|
Ash (g/kg) |
153 |
195 |
64 |
132 |
215 |
|
Crude protein (g/kg) |
244 |
241 |
337 |
364 |
297 |
|
Crude fibre (g/kg) |
136 |
124 |
129 |
133 |
198 |
|
Crude fat (g/kg) |
31 |
22 |
31 |
32 |
14 |
|
Nitrate (g/kg NO3) |
2.45 |
1.3 |
0.22 |
17.7 |
60 |
|
BC1 (g/kg Lactic ac.) |
90.4 |
70.7 |
21.6 |
36.3 |
22.7 |
|
WSC2 (g/kg) |
<10 |
<10 |
<10 |
48.1 |
15.1 |
|
WSC/BC Quotient |
0.11 |
0.14 |
0.46 |
1.33 |
0.66 |
|
FC3 |
6.53 |
6.67 |
8.73 |
20.2 |
10.5 |
|
DMmin4 (g/kg) |
517 |
610 |
587 |
336 |
383 |
|
End-products of the lactic acid fermentation |
|||||
|
DM (g/kg), fermented |
446 |
- |
430 |
404 |
395 |
|
pH |
4.04 |
- |
3.92 |
4.24 |
4.26 |
|
Lactic acid (g/kg) |
85.7 |
- |
80 |
86.8 |
74.2 |
|
Acetic acid (g/kg) |
4.3 |
- |
5.20 |
4.9 |
2.8 |
|
Butyric acid (g/kg) |
0 |
- |
0.6 |
0 |
0 |
|
Propionic acid (g/kg) |
0 |
- |
0 |
0 |
0 |
|
Alcohols4(g/kg) |
0.6 |
- |
2.9 |
0.4 |
0 |
|
Ammonia-N (g/kgtotal N) |
2.7 |
- |
0.3 |
1.10 |
9.5 |
|
Ammonia-N (g/kg CP) |
58 |
- |
5 |
16.0 |
164 |
|
DLG points5 |
100 |
- |
100 |
100 |
100 |
|
1 BC= Buffer Capacity |
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|
2 WSC= Water soluble carbohydrates |
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|
3 FC= Fermentability coefficient; FC>45, easily fermentable; FC from 35 to 45, medium fermentable; and FC<35, hardlyfermentable |
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|
4 Ethanol, methanol, n-propanol |
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|
5 DLG (Deutsche Landwirtschafts-Gesellschaft) guidelines for silage quality |
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|
Data corresponding to Spirodela polyrhiza were not analyzed for end-products of the fermentation |
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|
Table 2. Chemical composition of raw aquatic macrophytes used in Trial II (expressed on dry matter basis). |
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|
Chemical composition (g/Kg) |
Lemna minor |
Spirodela polyrhiza |
Azolla filiculoides |
E.crassipes(leaves) |
E.crassipes(stems) |
|
DM, fresh dry |
952 |
930 |
910 |
929 |
923 |
|
Ash |
270 |
241 |
258 |
167 |
251 |
|
Crude Protein |
157 |
212 |
198 |
192 |
97.8 |
|
Crude Fat |
22.5 |
22.5 |
17.1 |
33.0 |
25.5 |
|
Crude Fibre |
167 |
172 |
159 |
156 |
223 |
|
NFE1 |
384 |
353 |
368 |
452 |
402 |
|
GE2 (MJ/kg) |
11.4 |
12.2 |
11.9 |
13.9 |
10.4 |
|
Minerals (g/kg) |
|||||
|
Ca |
21.2 |
23.8 |
25.8 |
24.9 |
- |
|
P |
4.3 |
3.3 |
2.5 |
2.6 |
- |
|
Na |
17 |
14.5 |
22.8 |
3.5 |
- |
|
K |
25.5 |
22.2 |
15.2 |
24.6 |
- |
|
Mg |
17 |
15.1 |
22.9 |
4.1 |
- |
|
Zn (mg/kg) |
9.64 |
11.3 |
160.7 |
43.1 |
- |
|
Cu (mg/kg) |
4.34 |
8.81 |
14.81 |
7.14 |
- |
|
Cr (mg/kg) |
1.56 |
2.81 |
18.19 |
3.69 |
- |
|
Al (mg/kg) |
33.9 |
28.8 |
1.5 |
51.4 |
- |
|
Heavy metals (mg/kg) |
|||||
|
Cd |
0.48 |
0.76 |
1.31 |
0.53 |
- |
|
Ar |
N.d. |
N.d. |
N.d. |
N.d. |
- |
|
Se |
N.d. |
N.d. |
N.d. |
N.d. |
- |
|
Hg |
N.d. |
N.d. |
N.d. |
N.d. |
- |
|
Pb |
3.14 |
3.23 |
3.98 |
3.44 |
- |
|
N.d.: no detectable |
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|
1 Nitrogen-free Extract (NFE) = 100-(Ash+ Protein+ Fat + Fibre) |
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|
2Gross Energy (GE) calculated by 23.9 MJ/kg protein; 39.8 MJ/kg fat and 17.6 MJ/kg (NFE+CF) |
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The amino acid profile of tested local macrophytes and amino acids requirements of the tropical fish Nile tilapia (Oreochromis niloticus) and Pacu (Piaractus mesopotamicus) are presented in Table 4. The protein of the raw material resulted in a similar amino acid profile among plants and contained 5.30 to 6.28 g/100g lysine and 1.72 to 2.04 g/100 g methionine in the dietary protein. The tested aquatic macrophytes showed to be rich in aspartic acid and glutamic acid.
|
Table 3. Concentration of anti-nutritional substances in raw and fermented aquatic macrophytes (Trial II). |
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|
Anti-nutritional substances |
Lemna minor |
Spirodela polyrhiza |
A. filiculoides |
E. crassipes (leaves) |
||||
|
Raw |
Fermented |
Raw |
Fermented |
Raw |
Fermented |
Raw |
Fermented |
|
|
Trypsin inhibitor (mg/g) |
2.31 |
0.5 |
0.8 |
0.17 |
1.86 |
1.37 |
1.05 |
0.6 |
|
Phytates (% phytic ac.) |
0.32 |
0.12 |
0.25 |
0.11 |
0.15 |
0.15 |
0.15 |
0.12 |
|
Soluble tannins (%) |
0.3 |
N.d. |
1.31 |
N.d. |
0.44 |
N.d. |
0.7 |
N.d. |
|
Condensed tannins (%) |
N.d. |
N.d. |
3.87 |
N.d. |
N.d. |
N.d. |
0.99 |
N.d. |
|
Oxalates (%) |
2.02 |
0.04 |
0.1 |
N.d. |
1.67 |
0.19 |
0.52 |
0.1 |
|
N.d.: not detectable |
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|
Table 4. Amino acids profile of the aquatic macrophytes harvested from water bodies at northern Colombia (Trial II) and amino acids requirements (g/100g Dietary Protein) of common cultured tropical fish. |
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|
Amino acids (g 100g-1 Protein) |
Lemna minor |
Spirodela polyrhiza |
Azolla filiculoides |
E. crassipes (Leaves) |
Amino acids requirement |
|
|
Tilapia1 |
Pacu2 |
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|
Essential |
||||||
|
Arginine |
5.79 |
6.25 |
6.16 |
6.06 |
4.2 |
3.19 |
|
Histidine |
1.72 |
1.92 |
1.96 |
2.31 |
1.72 |
1.14 |
|
Isoleucine |
4.93 |
5.05 |
5.07 |
5.07 |
3.11 |
2.09 |
|
Leucine |
9.36 |
9.17 |
9.27 |
9.48 |
3.39 |
4.12 |
|
Lysine |
5.3 |
5.9 |
5.28 |
6.28 |
5.12 |
1.51 |
|
Methionine |
1.72 |
1.92 |
1.76 |
2.04 |
3.21 |
1.2 |
|
Phenylalanine |
5.54 |
5.47 |
5.62 |
6.12 |
5.59 |
2.06 |
|
Threonine |
4.93 |
4.69 |
5.07 |
4.79 |
3.75 |
2.07 |
|
Valine |
6.65 |
6.47 |
6.43 |
6.17 |
2.8 |
2.05 |
|
Tryptophan |
1.6 |
1.42 |
1.62 |
2.04 |
1 |
- |
|
Non-essential |
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|
Alanine |
7.64 |
7.04 |
6.83 |
6.61 |
- |
- |
|
Aspartic acid |
10.2 |
9.88 |
10.4 |
10.4 |
- |
- |
|
Cystine |
1.48 |
1.21 |
1.01 |
1.05 |
- |
0.37 |
|
Glutamic acid |
13.3 |
12.5 |
12.9 |
12.4 |
- |
- |
|
Glycine |
6.65 |
6.47 |
6.16 |
5.73 |
- |
- |
|
Proline |
5.17 |
5.4 |
5.14 |
5.18 |
- |
- |
|
Serine |
4.56 |
4.83 |
5.01 |
4.13 |
- |
- |
|
Tyrosine |
3.45 |
4.41 |
4.33 |
4.13 |
- |
1.72 |
|
1Nile Tilapia (Oreochromis niloticus), Santiago and Lovell (1988). 2Pacu (Piaractusmesopotamicus), Bicudo et al (2009). |
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The nutritional composition of the unfermented and fermented macrophytes is presented in Table 5. All tested variables showed significant differences at both factors except for ash content between treatments. The interaction between the plant species and treatments was significant and was not always in the same direction (disordinal interaction). Whereas crude fibre was significantly reduced (P < 0.05) in all fermented plants, crude protein varied among the plants species and resulted significantly higher (P < 0.05) in fermented Lemna and Spirodela and significantly lower (P < 0.05) in fermented Azolla and Eichhornia when compared to the respectively unfermented plant material. Ash content did not change.
|
Table 5. Nutrient composition (g/kg) of unfermented and fermented aquatic macrophytes (Trial II). |
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|
Experimental material |
Parameters |
||
|
Ash |
Protein |
Fibre |
|
|
Unfermented Lemna |
215 |
112 |
130 |
|
Unfermented Spirodela |
330 |
177 |
141 |
|
Unfermented Azolla |
299 |
190 |
118 |
|
Unfermented Eichhornia |
173 |
218 |
147 |
|
Fermented Lemna |
210 |
131 |
126 |
|
Fermented Spirodela |
322 |
184 |
104 |
|
Fermented Azolla |
339 |
163 |
102 |
|
Fermented Eichhornia |
166 |
210 |
143 |
|
Plants (P) |
Means |
||
|
Lemna |
213ab |
121a |
128a |
|
Spirodela |
326a |
181b |
123b |
|
Azolla |
319b |
176c |
110c |
|
Eichhornia |
169ab |
214d |
145d |
|
SEM |
3.99 |
0.72 |
1.06 |
|
Prob. |
0.001 |
0.001 |
0.001 |
|
Treatment (T) |
|
Means |
|
|
Unfermented |
254a |
174a |
134a |
|
Fermented |
259a |
172b |
119b |
|
SEM |
2.82 |
0.51 |
0.75 |
|
Prob. |
0.211 |
0.019 |
0.001 |
|
Interaction P x T |
|
|
|
|
Prob. |
0.001 |
0.001 |
0.001 |
|
Statistics |
Variables F values |
||
|
Plants (P) |
381 * |
2866 * |
184 * |
|
Treatment (T) |
1.70 NS |
6.79 * |
200 * |
|
Interaction P x T |
8.92 * |
187 * |
52.9 * |
|
NS= Not significant, * significant (P<0.05) |
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|
abcd Means in same column without common superscript are different at P<0.05 |
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A minimum WSC content of 75g/kg DM (Pahlow et al 2003) and an adequate amount of lactic acid bacteria are required to establish a good fermentation. The tested aquatic macrophytes presented a low WSC content (<50 g/kg DM), and additionally, a relatively high buffering capacity. They showed very low WSC/BC ratios and consequently low fermentation coefficients (FC<35). Therefore, the addition of molasses as source of WSC is required to improve fermentation. Likewise, as natural populations of lactic acid bacteria are often low in number and hetero-fermentative on the plant material producing end-products other than lactic acid (Ennahar et al 2003), the inclusion of LAB inoculants is also desirable to improve the silage potential of the tested aquatic macrophytes.
In fact, these components were applied and the amount of fermentation end-products in the aquatic macrophytes silages was comparable to those reported for common silages as grass, corn, and alfalfa. In general, the pH values were lower than 4.5 as recommended by DLG (2006), and lactic acid concentrations were closely related to those reported by Kung (2001) for good quality alfalfa silage (70-80 g/kg lactic ac.) and grass silages (60-100 g/kg lactic ac.). The DLG points obtained in this study indicated very good silage fermentation.
The nutritional composition of the raw aquatic macrophytes in trial II was characterized by a high ash and crude fibre content, a limited lipid content (17-33 g/kg), an acceptable protein content (160-210 g/kg DM) considering the requirement of fish, and a well balanced amino acid composition. The content of ash and fibre for the tested plants in this study was comparable with values reported for several aquatic plants by Bairagi et al (2002), El-Sayed (2003), Kalita et al (2007) and Leterme et al (2009). Low content of lipids was also reported by Bairagi et al (2002)for Lemna polyrhiza (15 g/kg) as well as by El-Sayed(2003) for Eichhornia crassipes (10 g/kg). In contrast, Kalita et al (2007) reported a highercontent of lipids for Lemna minor (50 g/kg) from northeast India when compared to the present study. The deficit of lipids should be supplemented by additional components when the aquatic macrophytes are included into fish diets.
The crude protein content of Eichhornia crassipes found in trial I differs from values found in literature and from the findings of trial II for which the plants were harvested in natural ecosystems. A higher nutrient content can be explained by the ability of Eichhornia to take up nutrients from the water. Mainly, this occurs when they grow in nutrient-rich water provided with large amounts of chemical nutrients as is usual for cultured aquatic plants as those used in trial I.
Aquatic macrophytes are rich in minerals, exceeding the fish requirements but not the critical values for fish. Mineral composition of the raw aquatic macrophytes revealed a comparable content among plants, except for Azolla. Concentrations of calcium and phosphorus were similar in all the plants. Calcium and potassium were the most abundant minerals tested. Phosphorus content in Lemna and Spirodela ranged within the requirements reported for common fin fish (NRC 1993), whereas the Ca:P ratio was higher than the fish requirements.The reduction of calcium in the mineral mixture used in formulated diets must be considered.
Azolla showed the highest amount of zinc (161 mg/kg), copper (14.8mg/kg) and chromium (18.2mg/kg). Although the requirement of zinc for the majority of fish is much lower, varying from 15 to 30 mg/kg (NRC 1993), higher levels of supplemental zinc are frequently included in the practical diets to compensate the reduced zinc bioavailability caused by other dietary factors such as phytates. In some fish species (trout and carp) the tolerable limit of zinc in diets has been reported as 1900 mg/kg (Jeng and Sun 1981; NRC 1993). Likewise, the requirement of copper for fish, which varies from 3 to 5mg/kg, is much lower than in the fern Azolla. However, it does not exceed the tolerable limit forfish diets, which has been reported as 150 mg/kg (NRC 1993). Mineral concentration should be considered before the inclusion of Azolla into fish diets depending on the fish species and its particular tolerable limits.
The heavy metal concentration is particularly important as aquatic plants tend to accumulate them. In this study, the concentrations of the heavy metals arsenic, selenium and mercury were not detectable. Cadmium ranged in very low amounts from 0.48 to 1.31 mg/kg, whereas lead ranged from 3.14 to 3.98 mg/kg. Cadmium has been reported to be absorbed through the gastrointestinal tract of fish (NRC 1993) and causes liver necrosis and mortality at doses of 5 mg/kg of body weight. In contrast, Hodson et al (1978) reported that dietary lead was not absorbed by rainbow trout fed lead in different amounts. In this study the concentrations of heavy metals were not critical, but if aquatic macrophytes were used as exclusive feed source for fish, heavy metal contamination of feed, particularly cadmium retention, must be considered since it reduces fish growth, feed conversion and can be toxic.
Except for phytates content in Azolla, the antinutritional substances, trypsin inhibitor, phytates,tannins(hydrolyzed and condensed), and oxalates were significantly reduced by the lactic acid fermentation. According to Francis et al (2001) the tolerable limit of trypsin inhibitor is below 5 g/kg TI for the most cultured fish. Likewise, phytates (as phytic acid) and sodium phytates have been reported to cause depression in growth and food conversion efficiency of fish at levels of 5 g/kg and 10 g/kg in diets (Spinelli et al 1983,Hossain and Jauncey 1993). The level of trypsin inhibitor (lower than 1.37 mg/g TI), phytates (lower than 1.5 g/kg phytic ac.), tannins (not detectable) and oxalate (about zero) in fermented aquatic macrophytes did not exceed the critical value for commonly cultured fish.
Crude fibre was significantly lower in the fermented aquatic macrophytes when compared to the unfermented samples. This decrease in the fibre content could be explained by the partial acid hydrolysis of hemicelluloses resulting from the microbial utilization (Jones 1975).Crude protein content was also affected by fermentation. However, the effects of lactic acid fermentation on the protein content are conditional and strongly depend on the plant species. Thus, changes can be explained by differences in the chemical properties of the plant species, by the effect of molasses supplementation, and by the processes occurred on the plant material over the six weeks of fermentation. The decreases of crude protein in fermented Azolla and Eichhornia may be related to a slower acidification in the silage leading to an increase in proteolysis (Cussen et al 1995), whereas the increases of crude protein in fermented Lemna and Spirodelamay have been occurred through microbial synthesis (Wee 1991).
In general, lactic acid fermentation is highly recommendable before the inclusion of aquatic macrophytes into fish diets. As high fibre content of plant ingredients has a negative impact on digestibility (De Silva et al 1990), the raw aquatic macrophytes would not be recommended as exclusive nutrient sources. However, aquatic macrophytes silages may be used for the partial replacement of protein sources or as mineral source for the supplementation of basic fish feed in farming. Further research must be addressed to evaluate the optimum dietary inclusion level of the tested aquatic macrophytes in fish diets and the effect of their inclusion on fish performance. The establishment of easy practicable fermentation methods on-farm should be considered for the inclusion of the silage into fish diets.
The first author gratefully acknowledgesthe PhD scholarship award of the German Academic Exchange Services (DAAD). The authors would also like to thank Prof. Dr. Richter for her support with statistical question marks, theWAKUS GmbH and the Botanical Garden of Berlinfor providing the plant material used in the Trial I, and to Dr. Pieper Technologie-und Produktentwicklung GmbH (Germany) for providing the commercial silage inoculants BIO-SIL® used in the experiments. This work was financially supported by project COLCIENCIAS Cod. 1117-452-21305 and the University of Magdalena.
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Received 14 March 2011; Accepted 17 October 2011; Published 4 November 2011