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Sukumaran P, Thevanathan R. Phycochemical Property of Pithophora Oedogonia (Mont). Wittrock With Special Reference to its Neutraceutical Significance. Biosci Biotechnol Res Asia 2009;6(1)
Manuscript received on : January 08, 2009
Manuscript accepted on : February 17, 2009
Published online on:  28-06-2009
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Phycochemical Property of Pithophora Oedogonia (Mont). Wittrock With Special Reference to its Neutraceutical Significance

Pamela Sukumaran1 and R. Thevanathan2

1Department of Botany, Women’s Christian College, Chennai - 600 006 India.

2Post graduate and Research Department of Botany, Presidency College (Autonomous) Chennai - 600 078 India.

ABSTRACT: Pithophora oedogonia is a common alga of clear stagnant waters forming dense mats. The alga is generally considered as a nuisance alga and has been extensively studies for its growth requirements and characteristics to suggest control measures. However, its phycochemical qualities are not known.The neutraceutical properties of the alga were evaluated and compared with Spirulina which is commonly used in neutraceutical products.

KEYWORDS: Phycochemical properties; Pithophora oedogonia (Mont). Wittrock; neutraceutical

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Introduction

Marine algae have been widely used for human consumption.  They are consumed as regular part of human diet.  In coastal China, since 1850 (Waaland, 1981,) and today they are eaten mainly in the Orient and the Pacific islands. Chapman and Chapman (1980) lists 160 species of sea weeds eaten by humans 25, chlorophyceae, 54, phaeophyceae and 81, rhodophyceae (South and Whittick, 1987).  Porphyra, Laminaria, Undaria, Gigantina and Chondrus are some of the most widely used marine algae as food.  Food value, flavour, colour and texture appear to favour’ the use of algae as food.  While the protein content is high in these algae, metabolizable carbohydrates are much less.  Nevertheless, these algae are an excellent source of vitamins including, vitamin C at levels equivalent to citrus fruits and vitamins A, D, B1, B12, E, Riboflavin, Niacin, Pantothenic acid and folic acid.  They also serve as trace elements for human nutrition  (Yamamoto et al., 1979)and free amino acid (  Arasaki et al., 1984; Dave et al., 1993; Thevanathan et al., 1993,  Tasneem Fatima et al., 1994; Selvi et al., 1999).

Neutraceutical or health food market is currently flooded with many algae products that include dried biomass or all extracts produced from chlorella (Lee, 1997; Yamaguchui, 1997;), Dunaliella (Avron and Ben-Amotz, 1992) and Spirulina (Vonshak, 1997).  The nutritional qualities of these algae have led to the development of microalgal biotechnology in the last 2 decades.  Considerable attention is now being directed at unicellular algae for the production of oils and fatty acids.  The use of algal oils containing long-chain polyunsaturated fatty acids (LCPUFAs) as nutritional supplements is given primary focus (Cohen et al., 1995; Behrens and Kyle, 1996) and algal sources are being identified for the presence of docosahexaenoic acid (DHA) and eicosaapentaenoic acid (EPA). The DHA is a dominant fatty acid in neurological and heart muscle tissues and sperm cells.  The fact that humans are not capable of synthesizing DHA de novo implies the dependency on adequate supply of DHA through dietary sources (Emken et al., 1994).  The fatty acid is also a conditionally essential nutrient during infancy (Innis, 1994; Makarides et al., 1995) and a number of nutritional and professional organizations including the World Health Organistion have recommended the inclusion of supplementary DHA in infant formula.  Dinoflagellates are looked upon as a source of DHA for use in infant formulas (Apt and Behrens, 1999).  Changes in EPA levels are known to significantly alter the coronary vascular status of individuals (Salem, 1989) and a number of algae have been proposed for the production of EPA (Cohen, 1990; Sukenik, 1991; Boswell et al., 1992; Molina et al., 1995; Tan and Johns, 1996) and used in nutraceutical products.  It has also been suggested that algae can serve as a source of genes involved in LCPUFA synthesis (Apt and Behrens, 1999).  Apart from DHA and EPA, Arachidonic acid and has also been shown to be an important component of nutritional supplements and algae serving as a source for the fatty acids(Zhang Cheng Wu et al.,2002).

The fast growing aqua culture industry is also dependent on algae from which the aqua culture animals must obtain all the nutrients and the nutrient properties of the algae are critical for the growth and survival of both larva and adults.  Many of the algae are cultured for use in aqua culture industries (Day et al., 1991; Orus et al., 1991; Johnson and An, 1991; Benemamm, 1992; Chaumont, 1993; De Roeck et al., 1993; Barclay et al., 1994; Gladue and Maxey, 1994; Kashiwakura et al., 1994; Renaud et al., 1994; Qiang and Richmond, 1994; Takeyama et al., 1996; Barclay and Zeller, 1996; Bret and Muller-Navarra, 1997; Borowitzka, 1997; Spektorova et al., 1997;Lynch, 1998;Vishwanath Patil et al.,2007).  The growing demand for safe natural products by the nutraceutical and aqua cultural industries has signified the importance of algae as a source of these products and the need to screen more algae for the purpose.  Very few fresh water algae have been screened for these nutritionally valuable products.

Pithophora oedogonia, the ‘horse hair’ or ‘cotton ball’ alga is a green alga that belongs to the family  Cladophoracea, order cladophorales of the class chlorophyceae.  The alga produces free floating mats of vegetation in static or slow moving bodies of water.  Its luxuriant growth in shallow lakes and ponds  biomass  production in huge quantities, high degree of resistance to copper and many algicides and occurrence as thick large clumps or mats with profusely branched  filaments having rigid, coarse cell walls have placed the alga in a prominent position as a filter clogging or nuisance alga of the water systems.  Though the alga has been studied as a nuisance alga, its nutritive and bioactive properties are not exploited.  The present investigations explores the possibilities of exploiting this alga in neutraceutical industries. The alga was screened for its mineral, aminoacid,vitamin, sterols and fatty acid content.

Materials and methods

The crude fiber content was estimated following the procedure of AOAC 1999. The ash content was analysed following  woodman 1945, Moisture and food energy (Gopalan 1989) and the total lipid content ( Bligh and Dyer 1959)The following minerals Sulphate, chloride, Phosphate, Sodium, Boron, Calcium, Magnesium and extractable metals such as Lead, Comium, Iron, Cupper, Cadmium, Nickle and Zinc were determined  (APHA 1989). The fatty acid content was analysed using Hewlett Packer GC model No: 5890. Aminoacid analysis was carried out on Beckman 119CL model automatic aminoacid analyzer (Arasaki 1984) αtocopherol  of the fresh and dry powdered sample was estimated by HPLC (Mallet et al. 1993 ). The vitamin was analysed according to AOAC 1990.  Extracted Sterols  from dry lipid preparations of the algal mats was separated identified and quantified by GC.

Results

Mineral and Biochemical Composition of Pithophora Oedogonia         

Mineral Composition

Dry powdered material of the alga was analysed for its mineral  and heavy metal composition (Table 1). The dry algal powder was found to contain the elements sodium, potassium, copper, iron, sulphate, phosphate, chloride, boron, calcium and magnesium. Of these elements, magnesium formed the bulk with 14.666 mg/g dry weight of the material. This is followed by sulphate with 9.9 mg/g and chloride with 9.73 mg/g dry weight of the alga. Potassium was present at a concentration of 6.45 mg/g dry weight. In addition to these heavy metals, lead, zinc, chromium, cadmium and nickel were present in the dry powder at detectable levels. Zinc was present at a concentration of 1.445 ppm, followed by chromium
(0.763 ppm), nickel (0.325 ppm) and lead (0.215 ppm) in the decreasing order (Table 1). Cadmium was present in trace amounts (less than 0.001 ppm).  The ash content of the dry powder was 34.75% and acid washable ash content was 16.19%. Total nitrogen level of the dry algal powder was 83.6 – 84.2 mg/g dry weight while the moisture content was 6.79%.  Fat content of the dry powder was 1.67% while that of protein was 20.5%. Crude fiber constituted 15.17% while the total carbohydrate content amounted to 21.12% of the dry powdered alga. Hundred grams of the dry material had a calorific value of 181.5.

Table 1: Mineral composition of P.oedogonia. 

Moisture   6.79 %
Ash 34.75 %
Acid washable ash 16.19 %
Protein  20.5 %
lipid  1.67 %
Crude fiber  15.17%
Total nitrogen 83.6-84.2mg
Sodium 2.24 mg/g
Potassium 6.45  mg/g
Copper 0.006 mg/g
Iron 0.198 mg/g
Sulphate  9.9 mg/g
 Chloride 9.73 mg/g
Phosphate 0.1626 mg/g
Boron 0.157 mg/g
Calcium 1.866 mg/g
Magnesium 14.676 mg/g
Heavy metals
Cadmium Trace
Lead 0.215ppm
Nickle 0.325ppm
chromium 0.763ppm
Zinc 1.445 ppm

Fatty Acid Composition

The fatty acid composition of the alga was estimated per unit lipid vide Materials and Methods. Thirteen fatty acids, namely undecanoic acid, lauric acid, tridecanoic acid, myristic acid, pentadecanoic acid, palmitic acid, heptadecanoic acid, stearic acid, arachidic acid, palmitoleic acid, oleic acid, cis-linoleic acid and arachidonic acid were detected in GC in the lipid sample of the alga (Table 2). Palmitoleic acid, oleic acid, cis-linoleic acid and arachidonic acid are the unsaturated fatty acids present in the sample and they constituted nearly 64% of the total fatty acid fraction.  cis-linoleic acid and the saturated arachidic acid formed the bulk of total fatty acids. Cis-linoleic acid alone constituted 50% of the total content while arachidic acid took a share of 26%. The rest of the fatty acids were present in quantities less than 6.0 mg/g.

Table  2: Fatty acid composition of  P.oedogonia.

S.No No. of carbon No.of double bonds    Fatty acid  Quantitymg/g  

 %

Sat/

unsat

   1.   11     0 Undecanoic acid     3.1873  2.73  Sat
   2.   12     0 Lauric acid     0.2755  0.23  Sat
   3.   13     0 Tridecanoic acid     3.7306  3.20  Sat
   4.   14     0 Myristic acid     3.1686  2.74  Sat
   5.   15     0 Pentadecanoic acid     1.6523  1.41  Sat
   6.   16     0 Palmitic acid     3.1361  2.69  Sat
   7.   17     0 Heptadecanoic acid     0.9815  0.84  Sat
   8.   18     0 Stiaric acid     4.6559  3.99  Sat
   9.   20     0 Arachidic acid     31.161  26.7  Sat
  10.   16     1 Palmitolic acid     0.5753  0.49 Unsat
  11.   18     1 Oleic acid     5.2328  4.49 Unsat
  12.   18     2 Cis linoleic acid     58.675 50.38 Unsat
  13.   20     4 Arachidonic acid     0.0224 0.019 unsat
Total    116.455

Amino Acid Composition    

The protein fraction of the alga showed the presence of 22 amino acids namely cysteine, ornithine, aspartic acid, glutamic acid, serine, glycine, asparagine, alanine, glutamine, histidine, lysine, arginine, proline, methionine, leucine, tyrosine, tryptophan, phenylalanine, threonine, valine, isoleucine and g-amino butyric acid (Table 3). Interestingly the amides asparagine and glutamine were found only in traces in the protein fraction. Aspartic acid constituted 22% of the proteins.  The other major components are glutamic acid (9.9%), leucine (7.7%), glycine (8.7% ), isoleucine (6.1%) and arginine (6.09%).

The free aminoacid pool showed the presence of only 20 amino acids of which tyrosine and tryptophan were present in trace amounts (Table 3). In contrast to that observed for protein amino acids, cysteine is the major component of the free amino acid pool comprising 22.4% of the total amino acid. The lysine constituted 10.6% of the total pool. The other major constituents are asparagine (12.2%) arginine (10.6 %) leucine (5.9%) and ornithine (5.7 %).

Table 3: Aminoacid composition of   P. oedogonia.

S.No    AMINO ACID PROTEIN AMINO

ACID

 

   FREE POOOL  

 

mg/g protein % Total mg/g fresh wt. % Total
1. Cystine 10.2 1. 48 126.8 22.4
2. Ornithine     –  31.7 5.62
3. Aspartate 150.3 21.9  18.2 3.22
4. Glutamic acid 66.3 9.6  15.4 2.73
5 Serine 34.1 4.9  12.7 2.25
6. Glycine 58.4 8.5  11.8 2.09
7. Asparagine Trace  69.2 12.27
8. Alanine 34.7 5.05  21.4 3.79
9. Glutamine Trace  15.8 2.8
10. Histidine 10.3 1.5  28.6 5.07
11. Lysine 28.6 4.16  60.0 10.64
12. Arginine 41.8 6.09  60.0 10.64
13. Proline 21.0 3.0  12.0 2.12
14. Methionine 10.0 1.4   9.2 1.63
15. Leucine 53.5 7.7  33.6 5.95
16. Tyrosine 22.0 3.2  Trace
17. Tryptophane Trace  Trace
18. Phenylalanine 38.4 5.59  19 3.36
19. Threonine 36.7 5.34  9.2 1.63
20 Valine 27.4 3.99    –
21. Isoleucine 42.3 6.16    –
22.  Amino butyric acid   9.2 1.63
Total amino acid 686 563.8

a-Tocopherol Content In Hexane Extract of Fresh and Dry Mats of P.Oedogonia

The hexane extracts of both fresh and dried mats of the alga were analysed for  a-tocopherol levels by HPLC. The analysis showed variations in the levels of a-tocopherol between the extract of dry and fresh material. Fresh extract contained 0.073% of a-tocopherol while the same in the extracts of dry mats was 0.09 %.

Vitamin Composition

Apart from a-tocopherol, vitamin A and vitamin B2 and other components of vitamin B complex were detected in sufficient levels
(Table 4).  Nicotinic acid, nicotinamide and ca-pantothenate were found in high levels. Nicotinic acid was present at 0.65 mg/g dry weight of the algal mats, while vitamin B2 was present at a concentration of 0.04 mg/g dry weight.  The levels of vitamin A per gram dry weight of the algal mats was in the range of 200 ± 17 IU.  From the values obtained for vitamin A, b-carotene level was calculated in the tissues.  Gram dry weight of the material contain 120.0 µg carotene.

Table 4: Vitamin composition of P. oedogonia.

S.no        Vitamin  Quantity mg/g
1.  Nicotinic acid 0.658
2. Nicotin amide 0.219
3 Ca- pantothenate 0.278
4. Vitamin B6 0.083
5. Folic acid 0.029
6. Vitamin B2 0.04
7. Vitamin A 200  1U
Β-carotene 120 µg

                     

 

Sterol Composition

Gas chromatographic analysis of the sterol showed the presence of four peaks  with retention time of 33.42, 35.22, 39.16 and 41.26 respectively under the analytical conditions described elsewhere.  Of the four sterol peaks, two with retention time 35.22 and 39.16 were identified as stigma sterol and b-sitosterol respectively.  The other two sterols were not identified and were present in quantities comparable to that of stigma sterol using the same standard. Stigma sterol was present at a concentration of 0.067 mg/g lipid while b-sitosterol was present at a concentration of 0.586 mg/g lipid.  The latter was the major sterol component of Pithophora oedogonia.

Discussion

Biochemical composition especially proteins, carbohydrates, lipids, amino acids, fatty acids and the composition of minerals and vitamins are vital in determining the nutritional status of the alga and its usefulness as a nutritional substitute.  Analysis of the dry powdered material for its mineral and heavy metal composition revealed the presence of heavy metals in the range of 0.001 – 0.763 ppm.  Zinc was present at 1.445 ppm level.  The moisture content was 6.79% and ash 34.75%. Protein and lipid constituted 20.5%, 1.67 % respectively.  The concentrations of other minerals are given in Table 1.  A comparison of the data obtained for Pithophora oedogonia with that reported for Spirulina is given in Table 5.  The comparison shows that protein content of Pithophora oedogonia is relatively much less as compared to Spirulina.  Nevertheless, the crude fiber content, low levels of sodium and high levels of potassium and iron favour Pithophora oedogonia also as a nutraceutical product.  In recent years, dried biomass or cell extracts produced from Chlorella (Lee, 1997; Yamaguchui, 1997) Dunaliella (Avron and Ben Amotz, 1992), and Spirulina (Vonshak, 1997) have dominated the neutraceutical market.  In the search for sources of cheap proteins, minerals and essential amino acids, filamentous algae have not received due attention like unicellular forms mainly because of the rigid cellulosic cell walls.  A thick cellulosic cell wall of untreated algae is indigestible by nonruminants.  However, with advancements made in post harvest processing technology in recent years, a rigid cellulosic cell wall may not pose a big problem for algae like Pithophora oedogonia.  Fiber content is very high in this alga and only the protein content is not to the level reported for unicellular forms.  Through genetic manipulations and selection techniques, it might be possible to increase the protein content of the alga in future.  However, it is only a theoretical possibility at present.

Table 5: A comparison of the Chemical composition of Pithophora oedogonia and Spirulina

Chemical P.oedogonia *Spirulina
 Moisture   6.79 %  7.0%
Ash   34.75 %  9.0%
Acid washable ash   16.19 % —–
Protein    20.5 %  71.0%
Lipid    1.67 %  7.0%
Crude fiber    15.17%  0.9%
Total nitrogen 83.6-84.2mg  !3.35%
Sodium   2.24 mg/g  412mg/kg
Potassium   6.45  mg/g 15400mg/kg
Copper   0.006 mg/g
Iron   0.198 mg/g 580mg/kg
Sulphate   9.9 mg/g
 Chloride   9.73 mg/g 4400mg/kg
Phosphate   0.1626 mg/g
Boron   0.157 mg/g
Calcium   1.866 mg/g 1315mg/kg
Magnesium  14.676 mg/g 1915mg/kg
Heavy metals
Cadmium   Trace >0.10ppm
Lead   0.215ppm 0.40ppm
Nickle   0.325ppm —-
Chromium   0.763ppm —–
Zinc  1.445 ppm 39mg/kg

 *  Source MCRC Hand book  ‘The wonder gift of nature’

Table 6: A comparison of the  amino acids of Pithophora oedogonia     and Spirulina*

S.no Amino acid P.oedogonia P.oedogonia

 amino acid

freepool

Spirulina
Protein amino acid
1. Cystine    1.4 8 % 22.49   3.46 %
2. Ornithine 5.62
3. Aspartate     21.9 % 3.22   6.43 %
4. Glutamic acid     9.66 % 2.73   8.94 %
5 Serine      4.9 % 2.25    4.0  %
6. Glycine      8.5 % 2.09   3.46 %
7. Asparagine 12.27
8. Alanine     5.05 % 3.79    5.82 %
9. Glutamine 2.8
10. Histidine     1.5 % 5.07   1.08 %
11. Lysine     4.16 % 10.64    4.0 %
12. Arginine     6.09 % 10.64   5.98 %
13. Proline      3.0 % 2.12   2.97 %
14. Methionine      1.4 % 1.63   2.17 %
15. Leucine      7.7 % 5.95    5.8 %
16. Tyrosine      3.2 %
17. Tryptophane   1.13 %
18. Phenylalanine      5.5 % 3.36   3.95 %
19. Threonine      5.34 % 1.63   4.17 %
20 Valine      3.9 9 %    6.0 %
21. Isoleucine      6.16 %   4.13 %
1.63

 * Source MCRC Hand book  ‘The wonder gift of nature’

Table 7: A comparison of the Fatty acids of Pithophora oedogonia  and  Spirulina*.

S.No Fatty acid P.oedogonia                          mg/Kg Spirulina          mg/Kg
   1. Lauric acid     275.5  229
   2. Myristic acid     3186 664
   3. Palmitic acid     3136 21,141
   4. Palmitolic acid     575.3 2565
   5. Heptadecanoic acid     981.5 142
   6. Stearic acid     4655.9 353
   7. Oleic acid     5232 3,009
   8. Cis- linoleic acid     58675 13784
   9. Undecanoic acid     3187
  10. Tridecanoic acid     3730
   11. Pentadecanoic acid     1652
  12. Arachidonic acid     22.4
   13 Arachidic acid     31161                       —

* Source MCRC Hand book  ‘The wonder gift of nature’

 **  value for P. oedogonia are per kg extractable lipid from    algal mats  Value for spirulina are for per unit dry weight of the alga

The amino acid analysis showed the presence of 20 amino acids.  Cystine, asparagine, lysine, arginine and leucine are found to occur in huge quantities (Table 3).  Levels of these amino acids are as high as compared to that reported for Spirulina and other SCP algae.  In Pithopora oedogonia lysine content is 10.64% in free amino acid pool and 4.16% in protein fractions as against 4% in the protein of Spirulina (Table 6).  Thus the amino acid composition is relatively better in Pithopora oedogonia as compared to Spirulina. Many amino acids such as leucine, lysine, aspartate, glutamate, glycine, phenylalanine, threonine, and arginine are present in Pithophora oedogonia in high levels as compared to Spirulina (Seshadri, MCRC hand book, Becker and Venkataraman 1982; Venkataraman, 1983).  Total lipid content of Pithophora oedogonia is 1.67% and it contained the fatty acids undecanoic acid, lauric acid, tridecanoic acid, myristic acid, pentadecanoic acid, palmitic acid, heptadecanoic acid, stearic acid, arachidic acid, palmitoleic acid, oleic acid, cis-linoleic acid and arachidonic acid (Table 2).  Available information on the fatty acid composition of Spirulina shows the presence of only lauric, myristic, palmitic, palmitoleic, oleic, heptadecanoic, stearic and cis-linoleic acids only in its dry powder preparations (Table 7).  It may be noted that the unsaturated fatty acids are present in high levels in Pithophora oedogonia as the data presented in this thesis for these fatty acids is per unit lipid as compared to that of  Spirulina. 

In recent years, considerable attention has been directed at algae for the production of oils and fatty acids and the use of algal oils containing long chain polyunsaturated fatty acids (LCPUFA) as nutritional supplements (Cohen et al., 1995; Behrens and Kyle, 1996; Apt and Behrens, 1999). The presence of arachidonic acid, a polyunsaturated fatty acid (20:4) in Pithophora oedogonia is an interesting and significant finding in this context. This fatty acid is a precursor of all eicosonoides and is involved in many vital physiological processes of human beings. Fatty acid and sterol composition is critical and distinct for an algal group and alga as well.  Sterol distribution shows greater promise as chemotaxonomic markers (Volkmann, 1986; Mansour et al., 1999).  Sterols induce a wide range of responses in plant and animal tissues.  Gas chromatographic analysis showed the presence of stigmasterol and b-sitosterol in Pithophora oedogonia. Beta-sitosterol is present at a concentration of 0.5861 mg/g while stigmasterol was at 0.067 mg/g.  Dry powdered material of the alga contained nicotinic acid (0.65mg/g), nicotinamide (0.219 mg/g), Ca-pantothenate (0.278 mg/g), Vitamin-A 200 IU, Vitamin B2 (0.49 mg/g), Vitamin B6  (0.83 mg/g) and folic acid (0.029 mg/g). Vitamin E as  a-tocopherol was 0.073% in the n-hexane extract of fresh mats and 0.09% in dry mats of the alga .

High crude fiber content, high levels of iron, ash, calcium and phosphate, low levels of heavy metals, presence of long chain poly unsaturated fatty acids constituting more than 50% of total fatty acid content, presence of arachidionic acid which is the precursor of all eicosonoides, occurrence of essential amino acids in large quantities, presence of vitamins in levels comparable to that reported for Spirulina especially of vitamin E, and the high antioxidant potential of the alga suggest that Pithophora oedogonia could serve as a better substitute,  if not the best for many available neutraceutical products.  Lesser protein as compared to other products and the rigid cellulosic cell wall may be disadvantageous for the alga to be commercially exploited for neutraceutical purposes. However, proper post harvest processing technology, genetic manipulation and selection techniques might help in overcoming these disadvantages. Biochemical composition especially proteins, carbohydrates, lipids, amino acids, fatty acids and the composition of minerals and vitamins are vital in determining the nutritional status of the alga and its usefulness as a nutritional substitute.  Analysis of the dry powdered material for its mineral and heavy metal composition revealed the presence of heavy metals in the range of 0.001 – 0.763 ppm.  Zinc was present at 1.445 ppm level.  The moisture content was 6.79% and ash 34.75%. Protein and lipid constituted 20.5%, 1.67 % respectively.  The concentrations of other minerals are given in Table 1.  A comparison of the data obtained for Pithophora oedogonia with that reported for Spirulina is given in Table 5.  The comparison shows that protein content of Pithophora oedogonia is relatively much less as compared to Spirulina.  Nevertheless, the crude fiber content, low levels of sodium and high levels of potassium and iron favour Pithophora oedogonia also as a nutraceutical product.  In recent years, dried biomass or cell extracts produced from Chlorella (Lee, 1997; Yamaguchui, 1997) Dunaliella (Avron and Ben Amotz, 1992), and Spirulina (Vonshak, 1997) have dominated the neutraceutical market.  In the search for sources of cheap proteins, minerals and essential amino acids, filamentous algae have not received due attention like unicellular forms mainly because of the rigid cellulosic cell walls.  A thick cellulosic cell wall of untreated algae is indigestible by nonruminants.  However, with advancements made in post harvest processing technology in recent years, a rigid cellulosic cell wall may not pose a big problem for algae like Pithophora oedogonia.  Fiber content is very high in this alga and only the protein content is not to the level reported for unicellular forms.  Through genetic manipulations and selection techniques, it might be possible to increase the protein content of the alga in future.  However, it is only a theoretical possibility at present.

Easy availability of the alga, simple growth requirements and fast growth under enriched conditions are added advantage for exploitation of the alga commercially as a neutaceutical substitute. The findings presented in this paper would certainly form a basis to view Pithophora oedogonia, the ‘nuisance alga’. as a potential source of biologically active natural products for neutraceutical application.

References

  1. AOAC. 1999. Official methods of analysis, 16thed. Association of  official analytical chemists, Washington.D.C.
  2. Apt, K.E. and Behrens, P.W. 1999. Commercial developments in microalgal biotechnology. Phycol. 35 : 215 – 226.
  3. Arasaki, F.T., Norikomino and Mitsuekuroda. 1984. The protein value in human nutrition of edible marine algae in Japan. Hydrobiologia 116/117 : 513 – 516.
  4. Avron, M. and Ben-Amotz, A., Eds. 1992. Dunaliella: Physiology, Biochemistry and Biotechnology. CRC Press, Boca Raton, Florida . 240 pp.
  5. Barclay, W and Zeller.S. 1996. Nutritional enhancement of n- 3 and n- 6 fatty acids in rotifers and Artemia nauplii by feeding spray dried Schizochytrium sp. J.World Aquacult. Soc.  27 : 314 – 322.
  6. Barclay, W.R., Meager, K.M., and Abril, J.R. 1994. Heterotrophic production of long chain omega- 3 fatty acids utilizing algae. Appl. Phycol. 6 : 123 –129.
  7. Becker, E.W. (Ed.) 1994. Microalgae: Biotechnology and Microbiology. Cambridge Studies in Biotechnology, vol. 10, Cambridge University Press, Cambridge, 239 pp.
  8. Becker, E.W. and Venkataraman, L.V.  1982. Biotechnology and exploitation of algae. An Indian approach. pp.216.
  9. Behrens, P.W. and Kyle, D.J. 1996. Microalgae as a source of fatty acids. Food lipids. 3 : 259 – 272.
  10. Bennemann, J.R. 1992. Microalgae aquaculture feeds. Appl. Phycol. 4 : 233 – 245.
  11. Bligh, E.G. and Dyer, W.J. 1969. A rapid method of total lipid extraction and purification. Can .J. Biochem. Physiol. 37 : 911–917.
  12. Boswell, K.D.B., Gladue, R., Prima, B.  and Kyle, D. J. 1992. SCO production by fermentative microalgae. In Kyle, D.J. & Ratledge, C. (Eds.) Industrial Application of Single Cell Oils. American Oil Chemist society, Champaign, Illinois, pp 274-286.
  13. Brett, M.T and Müller-Navarra. 1997. The role of highly unsaturated fatty acids in aquatic food web processes. Fresh Water Boil. 38 : 483 – 499.
  14. Borowitzka, M.A. 1997. Micro algae for aqua culture: Opportunities and constraints. J.Appl. Phycol. 9 : 393 – 401.
  15. Chapman, V.J. 1970. Sea weeds and their uses 2nded Methuen , London 304 pp.
  16. Chapman, V.J and Chapman, D.J. 1980. Seaweeds and their uses. Chapman and Hall London and NewYork.
  17. Chaumont, D. 1993. Biotechnology of algal biomass production. A review of systems for outdoor mass culture. Appl. Phycol. 5 : 593 – 604.
  18. Cohen, Z. 1990. The production potential of ecosapenaenoic acid arachidionic acid by red alga Porphyridium cruentum. J.of Am. Oil. Soc. 67 : 916 – 920.
  19. Cohen, Z., Norman, H.A. and Heimer, Y. M. 1995. Microalgae as a source of omega –3 fatty acids. World Rev. Nutr. Diet. 77 : 1–31.
  20. Dave, M.J. and Chauhan, V.D. 1993. Seaweed as a source of food feed and fertilizer. Invention intelligence  24 (3) : 115 – 121.
  21. Day, J.G., Edwards, A.P. and Rodgers, G.A. 1991. Development of an industrial scale process for the heterotrophic production of micro- algal mollusc feed. Bioresource Technol. 38 : 245 – 249.
  22. De Roeck Holtzhauer, Y., Claire, C., Bresdin, F., Amicel,  l. and Derrien, A. 1993. Vitamin free amino and fatty acid composition of some marine  planktonic microalgae used in aquaculture. Bot. Mar. 36 : 321– 325.
  23. Emken, F.A., Adolf, R.O. and Gulley, R.M. 1994. Dietry linolenic acid influences desaturation and acylation of deuterium labeled linoleic and linolenic acids in young adult males.Biochem. biophys. Acta.1213 : 277-288.
  24. Glaude, R.M. and Maxey, J.F. 1994. Microalgal feeds for aquaculture. Appl. Phycol. 6 : 131– 141.
  25. Gopalan, G., Rama Sastri, B.V., Balasubramanian ,S.C. 1989. Nutritive value of Indian foods. National institute of nutrition . Hyderabad.
  26.  Kashiwakura, M., Seto, A.  and Hasegawa, K. 1994. Hetertrophic macroalgal production of decosahexaenoic acid (DHA) and its use for aquaculture of marine Juvenile fish. Third international marine biotechnology conference. May, Baltimore. MD.p.61
  27. Innis, S.M. 1994. Fatty acid requirements of the new born. J.Physiol.Pharmacol. 72 : 1483 – 1492.
  28. Lee, Y.K. 1997. Commercial production of microalgae in the Asia Pacific rim .           Appl. Phycol. 9 : 403 – 411.
  29. Lynch, R. 1998. Aquasearch delaying kan expansion deal.Honolulu star Bulletin 1998-06-19:CA
  30. Mallet, J.R., Debel, A., Vacciani, E., Guilliand, M and Gruber, M. 1993.
  31. Lipides foliaires 1. Tocopherols Francaisdiscorps Gras Etude et R Rechercheno 3: 175
  32.  Makridas, M., Neumann, M., Simmer, K., Pater, J. and Gibson, R. 1995. Are long chained polyunsaturated fatty acids essential nutrients in infancy? Lancet 345 : 1463 – 1468.
  33. Mansour, M.P., John K. Volkman, Anne E. Jackson and Susan I. Blackburn. 1999. The fatty acid and sterol composition of five marine dinoflagellate. Phycol. 35 : 710-720.
  34. Molina Geima, F., Sanchez Perez, J.A., Garcia Camacho, F., Fernandez sevilla, J.M., Acien Fernandez, F.C. and urda caedona, J. 1995. Biomass and icosapentaenoic acid productivities from an out door batch culture of Phaeodactylum tricornutum UTEX 640 in an airlift tubular photobioreactor. Appl.Microbiol. Biotecnol. 42 : 658 – 663.
  35. Qiang, H. and Richmond, A. 1994. Optimizing the population density in Isochrysis galbana grown outdoors in a glass column photo bioreactor. Appl.Phycol.6 : 391–396.
  36. Renaud, I.A., Parry, D.I. and Thinh, I.V. 1994. Microalgae for use in tropical aqua culture. 1. Gross chemical and fatty acid composition of twelve species of microalgae from the northern territory .  Australia. J. appl. Phycol.6 : 337-345.
  37. Renn, D. 1997. Biotechnology and the red seaweed polysaccharide industry: status, needs and prospects. Trends Biotechnol. 15 : 9-14.
  38. Salem. 1989.Omega 3 fatty acids : Molecular and biochemical aspects. In spiller, G. and Scala, J. (Eds) New protective roles for Selected Nutrients: Current topics in nutrition and disese, Vol 22 Alan R. Leiss New York pp 109 –228
  39. Selvi, M.  Shakila, P. and Selvaraj, R. 1999.Studies on bochemical content of macroalgae from Cuddalore and Tirumullaivasal estuaries of Tamil Nadu. Seaweed Res. Utiln. 21(1&2): 99 – 103
  40. Seshadri, C.V. and Seshagiri, S. Spirulina “ The Wonder Gift of Nature’.  Shri AMM Murugappa Chettiar Research Center.
  41. South,R.G. and Whittick, A. 1987. Introduction to Phycology. Blackwell scientific publication. Oxford. 341pp.
  42. Spectovora, L., Cresswell, R.L. and Vaughan, D. 1997. Closed tubular cultivators: an innovative system for commercial culture of microalgae. World Aquacult. 28 : 39 – 43.
  43. Standard Methods for the examination of water and waste water. 1989. 17 Ed. Ed.by Lenores Clesari, Arnold, E. green Berg, Rhodes Trussell, R. American public health associaion. Washington DC.
  44. Sukenik, A. 1991. Ecophysiological consideration in the optimization of eciosapentaenoic acid production by Nannochloropsis sp. (Eustigmatophyceae). Bioresour. Technol. 36 : 263 – 270.
  45. Tan, C.K. and Johns, M.R. 1996. Screening of Diatoms for heterotrophic eicosapentaenoic acid production. Appl. Phycol. 8 : 59 – 64.
  46. Takeyama. H., Iwamoto, K., Hata, S., Takano and Matsunaga,T.  1996. DHA enrichment of rotifers: A simple two step culture using the unicellular algae Chlorella reqularis and Isochrysis galbana. J. Mar. Biotechnol. 3: 244 – 247.
  47. Tasneem Fatima, Sarada, R and Venkataraman, L.V. 1994. Evaluation of selected strains of Spirulina for their constituents.  Phykos 33 (1&2) : 89 – 97.
  48. Thevanathan, R. Gangadharan, A and veerabadran, V. 1993. Role of cystine in algal nitrogen metabolism. Seaweed Res. Utiln. 16(1&2) : 1– 12.
  49. Venkataraman, L.V. 1983 A monograph on Spirulina Platensis. Biotechnology and applications. CFTRI. Mysore.
  50. Vishwanath Patil, Torsten Källqvist, Elisabeth Olsen, Gjermund Vogt and Hns R. Gislerød.2007Fatty acid composition of 12 microalgae for possible use in aquaculture feed.Aqua culture international.15:1-9.
  51. Vonshak, A. (Ed). 1997. Spirulina platensis (Arthrospora): Physiology, Cell biology and Biotechnology. Taylor and Francis ,London 233pp.
  52. Volkman, J.K. 1986. A review of sterol markers for marine and terrigenous organic matter. Org. Geo chem. 9 : 83 – 99
  53. Waaland,J.R. 1981. Commercial cultivation. In the Biology of seaweed (eds. Lobban,C.S. and Wynne, M.J.). pp726-741. Blackwell scientific publication, Oxford.
  54. Woodman, A.G., 1945.  Food Analysis. 4 ed. Page 23.
  55. Yamaguchi, K. 1997. Recent advances in microalgal bioscience in Japan, with special reference to utilization of biomass and metabolites. Appl.Phycol. 8 : 487– 502.
  56. Yamamoto, T., Yamaoka,T., Tuno, S., Tokura, R., Nishimura, T. and Hirose, H. 1979. Microconstituents in seaweeds. Proc. Int. seaweed Sym. 9: 445 – 450.
  57. Z Cheng-Wu, Z Cohen, I Khozin-Goldberg, A Richmond 2002. Characterization of growth and arachidonic acid production of Parietochloris incisa comb. nov ( … Journal of Applied Phycology.14;453-460
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