Department of Biochemistry and Molecular Biology
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- ItemOpen AccessArchachatina (Calachatina) Marginata Haemolymph Proteins, Physicochemical Characterization of Protein B.(Obafemi Awolowo University, 1985) Binutu, Olaoluwa Olujare; Aboderin, A.The haemolymph of Archachatina (Calachatina) marginata has been found to contain other proteins apart from the predominant protein, haemocyanin. One of the other protein components, Protein B, was isolated and purified using preparatory ultracentrifugation and gel filtration techniques. Physicochemical characterization, employing different techniques has showed that Protein B is different from the haemocyanin (and/or its subunit(s)) from this mollusc. Protein B has a molecular weight of 360KD consisting of two chains which are of identical molecular size. Amino acid composition for Protein B shows that: (i) there exist more acidic residues combined than those of the basic residues combined. (ii) there is a very large occurence of Proline residues (iii) there is also a large amount of cysteine residues. There is one gram atom of copper per dimer. Protein B is a glycoprotein. The carbohydrate portion is made up of units of acetylglucosamine and galactosamine. Peptic peptide fractionation of reduced carboxymethylated Protein B has shown that most of the carbohydrate can be found on a peptide having a mass of 15KD.
- ItemOpen AccessThe Catalytic Properties of the Isoenzymes of Glutathione Transferase from Fruit Bat, Eidolon Helvum (Kerr) Liver(2015-06-26) Ejim-Eze, Emmanuel EmekaThis study investigated the physiochemical and catalytic properties of the isoenzymes of glutathione transferase (GST) in the fruit bat (Eidolon helvum, Kerr) liver, with a view to having an understanding of the survival strategy of this animal, which feeds on various plant materials many of which contain toxic secondary metabolites. A 15% homogenate (15 g in 85 ml buffer) of a fresh liver sample, obtained from live bats, was prepared in 10 mM Tris-HCI buffer pH 8.0, containing 1 mM EDTA, 1 mM 2-mercaptoethanol and 10% glycerol, using a warring blender. The crude homogenate was centrifuged at 20,000 rpm for 30 minutes at 4°C using a Beckman ultracentrifuge to obtain a cloudy supernatant. The supernatant was further centrifuged at 45,000 rpm for 1hr to obtain a clear crude enzyme extract. The extract was purified on DEAE-Sephacel anion exchange chromatography and CM-TrisacryI cation exchange chromatography, followed by gel filtration on Sephadex G-100. Determination of native and subunit molecular weights of the purified enzyme was carried out by gel filtration on Sephadex G-100 and sodium dodecyl sulphate-polyacrylamide gel electrophoresis (SDS-PAGE) respectively. In order to classify the various purified GST isoenzymes obtained, the specific activities towards various substrates [1,2-dichloro-4-nitrobenzene (DCNB), 1-chloro-2,4-dinitrobenzene (CDNB), 1,2-epoxy-3-(p-nitrophenoxy)propane (EPNP), ethacrynic acid, 4-chloro-7-nitrobenzo-2-oxa-1,3-diazole (NBD-CI) and p-nitrophenyl acetate (p-NPA)] were determined by monitoring the enzyme-catalyzed conjugation of the various substrates with reduced glutathione (GSH} in a spectrophotometer under standard conditions. The apparent Michealis-Menten constant (Km) and maximal velocity (Vmax) for GSH, and some of the utilizable electrophilic substrates, were also determined by varying the concentrations of the substrates while keeping that of GSH constant and vice-versa. The data also obtained were analyzed by double reciprocal plot. Similarly, the effect of the inhibitors: cibacron blue, hematin, and S-hexylglutathione, which could be used to discriminate between the different GST classes were studied by assaying the enzyme at different concentrations of the inhibitors. The results showed that the DEAE-Sephacel anion- exchange chromatography resolved the crude enzyme extract into two major peaks of activity designated as A and B which were separately pooled. Further purification of pool A on CM-Trisacryl cation-exchange chromatography resolved it into four peaks of activity which were designated, following the established convention, as AA, AB, AC and AD; AA being the isoenzyme that eluted at the highest ionic strength and AD, the lowest. However, further purification of pool B on this column gave only one peak of GST activity, which was designated as isoenzyme B. The native molecular weight of the isoenzymes estimated from a calibration curve ranged from 40 to 44 kDa. The subunit molecular weights of each of the isoenzymes estimated by SDS-PAGE were between 21 to 23 kDa. On the basis of this, the native isoenzymes could therefore be said to be dimeric proteins. The fruit bat GST isoenzymes conjugated CDNB, NBD-CI and p-NPA to varying degrees with GSH, but could not utilize ethacrynic acid, DCNB and EPNP. Hematin inhibited all the isoenzymes to the same extent, but isoenzymes AB, AC and AD were more sensitive to cibacron blue than isoenzymes AA and B. In conclusion, the occurrence of GST in multiple forms with different catalytic properties could assist fruit bats in detoxication of various allelochemicals encountered during feeding.
- ItemOpen AccessA comparative biochemical study of the interaction of some trypanocides with rat tissue cellular systems(Obafemi Awolowo University, Ile Ife, Nigeria, 1986) Akanji, Musbau Adewumi; Edwin.O. Ngaha, J.O. FolahanThe effects of three trypanocides (tryparsamide, novidium and berenil) on rat liver and kidney were studied with a view to understanding the site of primary injury to the cell resulting from their administration. Four enzymes which are exclusively located in specific regions of the cell were used to monitor the regions affected by the drugs. The results obtained showed that administration of each of the three drugs resulted in massive increase of alkaline phosphates activity and a very marked inhibition of lactate dehydrogenase activity in both tissues. There was no significant effect on the lysosomal enzymes both in vivo and in vitro. These results indicate that tryparsamide, novidium and berenil ellicit their action on the cellular system of both liver and kidney in similar ways when administered to rats. Inhibition of lactate dehydrogenase activity which is located in the soluble fraction of cytoplasm may lead to accumulation of pyruvate in the cell. The massive increase of alkaline phosphates activity in the tissues may also lead to indiscriminate hydrolysis of phosphate esters needed for vital activities in the cell.
- ItemOpen AccessIncidence of Urinary Tract Infection (UTI) Among Pregnant Women in Ile-Ife, Nigeria(2015-03-18) Adebayo, Oluwabanwo JamesThis study investigated the incidence of urinary tract infection among pregnant women. It determined the current microbial isolates that are responsible for infection as well as their susceptibility to antibiotics. The period or trimester when pregnant women are prone to urinary tract infection and the age range when infection is prevalent were also determined, this was with a view to providing information that will prevent complications in pregnancy arising from urinary tract infection. Urine samples were obtained from 300 randomly selected pregnant women attending the Antenatal Clinic of Obafemi Awolowo University Teaching Hospital Complex Ile Ife. Each patient was given a sterile, wide-necked, leak proof container and requested to give 10-20ml sample of mid-stream urine with little or no contamination and provide information on the month or term of pregnancy. The samples were then labelled with the date, the name of the patient and time of collection. Thereafter the specimen was transferred to the laboratory. The freshly collected clean-catch midstream urine was mixed by gently rotating the container . Using a sterile calibrated wire loop that holds 1/1000 ml (0.001 m1), a loopful of urine was inoculated into cystine lactose electrolyte-deficient (CLED) agar, chocolate agar and MacConkey agar. The plates were then incubated at 37°C for 24 hours. The organisms that were isolated from colonies on these media were subsequently identified and characterized using various biochemical tests, while their antibiotic sensitivity patterns were determined using the agar-disc diffusion method. This result showed that 34.3 % of pregnant women examined had significant bacteriuria suggestive of UTI. The most frequent isolate was Escherichia coli (41.7 %), followed by Staphylococcus aureus (26.2 %), Klebsiella spp. (8.7 %), Proteus mirabilis (6.8 %), Candida albicans (9.7 %), Pseudomonas aeruginosa (2.9 %) and Streptococcus faecalis (3.9 %). Urinary tract infection was common in the last trimester of pregnancy among the younger age group of 17 to 26 years. Antibiotic sensitivity tests showed that the Gram negative isolates were sensitive to nitrofurantoin, gentamicin, nalidixic acid and ofloxacin, while the Gram-positive isolates were sensitive to gentamicin, erythromycin and cloxacilin. High antibiotic resistance was observed by the urinary bacterial isolates to most of the antibiotics used, these however cannot be referred to as multiple antibiotic resistance. Klebsiella spp, P. mirabilis, P. aeruginosa and S. aureus were resistant to the following antibiotics, amoxycillin, cotrimoxazole, augmentin and tetracycline. E. coli was resistant to amoxicillin and cotrimoxazole while S. faecalis showed strong resistance to tetracycline. The study concluded that the leading microbial strains responsible for urinary tract infection among pregnant women at Ile Ife were Escherichia toll, Klebsiella and Staphylococcus aureus and most of the isolates were sensitive to nitrofurantoin, gentamicin and nalidixic acid.
- ItemOpen AccessInduction of Interferon by Poly A: Poly U in Primary Tissue Cultures.(Obafemi Awolowo University, 1985) Chujor, Chujor Samuel Nwafor; Folahan, J. O.Primary tissue culture was grown using bat (Eidolon helvum) breast muscle. These tissue cultures were treated with polyadenylic acid: polyuridylic acid) polyA: polyU). After 24 hours the culture brew was harvested and from this, interferon was extracted and purified to a specific activity of 1.5 x 105 IFN Units/mg protein. The interferon was shown to have a molecular weight of 24,000 and fully protected bats' cells from the action of Wesselsbron Virus (H10964).
- ItemOpen AccessInteractive Roles of Terpenoid Extract from the Leaves of Neem Plant (Azadirachta Indica A. Juss) On Lead-Induced Toxicity in Pregnant Rabbits(2015-06-19) Areola, Jacob OladayoThis study extracted terpenoid from the dried leaves of Neem plant (Azadirachta indica,A.JUSS). It also assessed the possibility of ameliorating the toxic effects and accumulation of lead in both the mother and the litters. This was with a view to investigating its interactive roles in lead-induced toxicity in pregnant rabbits and resulting litters. Fresh leaves were collected from Azadirachta indica trees planted on Obafemi Awolowo University campus, Ile-Ife, Nigeria. The leaves were air dried for 21 days and milled to fine powder. Terpenoid was extracted from dried leaves of Azadirachta indica by a procedure that consisted of solvent extraction with methanol (7.2 L), liquid-liquid partitioning with petroleum ether and ethyl acetate and evaporated under reduced pressure. The residue was phytochemically screened for terpenoids. Pregnant rabbits (does) weighing between 3.0 and 3.4 kg were randomly divided into 4 groups. Group I served as control and were treated orally with olive oil (2 ml/kg body weight per day). Group II served as Lead control and were treated with Lead acetate solution (50 mg / kg body weight per day). Group III served as positive control and were treated with ascorbic acid (400 mg / kg body weight per day) and Group IV served as terpenoid treated group and were treated with terpenoid extract (300 mg / kg body weight per day). One hour later, Lead acetate solution (50 mg / kg body weight per day) was administered to animals in groups III and IV. The animals were treated for 11 days starting from day 14 of pregnancy. The does and the litters (young rabbits) were sacrificed 4 weeks after parturition. Blood was collected into tubes containing anti-coagulants for plasma preparation while the blood for Lead analysis was collected into tubes without anticoagulants. Then, liver, kidney, heart and lungs were removed aseptically. The tissues were digested with (Conc.HNO3 : HC1 1 : 4 v/v) and portion of the liver was homogenized in phosphate buffer (100 mM, pH 7.4). Lead concentration in the tissues were determined by Atomic Absorption Spectroscopy (AAS). The total protein concentration in the plasma and liver homogenates were determined using biuret reaction method. The plasma albumin concentration was estimated as described in Sigma Chemical Limited catalogue. Hepatic marker enzymes (Alanine aminotransferase (ALT) and Aspartate aminotransferase (AST) activities were also determined spectrophotometrically at 505nm. The results revealed that, 15.8 g of terpenoid was obtained from 2.4 kg of dried leaf of neem plant representing 0.66% of the starting material. A total number of 32 litters were produced by pregnant rabbits in all the groups. There was no abortion and deformity of litters through out the duration of the experiment. The terpenoid extract was able to reduce Lead concentration in the blood, liver and kidney of pregnant rabbits by 45.45%, 30% and 20.9% respectively. The level of Lead reduction was found to be statistically significant (t = 3.365, p<0.05) but the extract had no significant effect on its concentration in the tissues of the litters. Lead concentration in terpenoid treated group was significantly lower than lead treated group (t = 3.365, p<0.05). All other parameters (Liver protein, plasma protein and albumin concentration, ALT and AST activities) were not significantly different in all the groups (t = 3.365, p>0.05). In conclusion, the terpenoid extract from the leaf of Azadirachta indica was not teratogenic and toxic to rabbits at the dosage used in these investigations. The extract was also able to reduce the lead burden in pregnant rabbits but could not produce the same effects on the litters.
- ItemOpen AccessProteins, Nature's Versatile Devices(Obafemi Awolowo University Press, 1981-02-17) Aboderin, A.It is our intentions in this lecture to explore some of the unities that characterise life from the intellectual niche of the protein molecule. To the extent that it can be demonstrated that the choice is not a parochial one, but one that belongs, if not at the centre, close to the centre of the phenomenon of life, to that extent will the intention of this discourse have been fulfilled. As is usual in this type of setting however it is fit and proper for me to seek the understanding of both the initiates and the laity, obviously for very different but understandable reasons. Proteins, as nature's versatile devices, function within comparatively macroscopic entities known as cells. As all students of biology and the history of biology are aware, the cell is the basic unit of biological life. As everyone again is aware there are different kinds of cells, In multicellular organisms such as the present lecture, there are brain cells, liver cells, kidney cells, all of which, within the proper observational grid, not only look different but also have different properties and functions.
- ItemOpen AccessPurification and Characterisation of Lectin from Bowringia Miladbraedii Harms Seeds(Obafemi Awolowo University, 1985) Alakija, Augusus Adegbolamiyo Olufemi; Animashaun, T.; Aboderin, A.A.Lectin was extracted from Bowringia mildbraedii Harms seeds and shown to agglutinate red blood cells nonspecifically. The chromatography using different grades of Sephadex did not give a very good separation of the lectin. Purification of the lectin by Sepharose 68 chromatography followed by metal chelate affinity chromatography was compared with purification by Sepharose 6B followed by ion-exchange chromatography using DEAE cellulose. The latter method was preferred and yielded a protein which behaved as a single protein on polyacrylamide gel electrophoresis. It was deduced that the lectin occured as a tetrameric protein with two subunits A and B having approximate molecular weight of 14,000 and 16,000 respectively from experiments with SOS-PAGE in the presence of 2, β-mercaptoethanol. The molecular weight of the lectin is approximately 60,000. The B. mildbraedii lectin precipitated Afzelia africana polysaccharide with remarkable specificity and failed completely to form precipitin bands in agargel double diffusion plates with other polysaccharides tested even at varying concentrations. The haemagglutinating and polysaccharide precipitating activity of the lectin is appreciably inhibited by µ-methylD-mannoside, D-mannose and D-glucose.
- ItemOpen AccessPurification and Characterization of Lectins from Abrus Species.(Obafemi Awolowo University, 1985) Caiquo, Aspect Wallace Kyemenu; Animashaun, T.Saline extracts prepared from Abrus precatorius and Abrus fructiculosus seeds agglutinated red blood cells. The agglutination was inhibited by D-galactose and lactose. The lectins bound to Sepharose 6B and were eluted with D-galactose. These lectins were separated into an agglutinin and a toxin by chromatography on Diethyl amino ethyl (DEAE) cellulose. The toxin from Abrus fructiculosus seed was named fructin' to distinguish it from Abrus precatorius seed toxin, abrin. In sodium dodecyl - polyacrylamide gel electrophoresis, (SDS-PAGE) fructin and abrin gave single bands with molecular weights (proposed) 60,320 and 62,500 respectively. After treatment with mercaptoethanol, fructin and abrin were split into 2 bands each with molecular weights 32,360 and 30,200 (fructin), 36,520 and 28,800 (abrin). The agglutinins gave 2 bands each in SDS-PAGE with corresponding molecular weights of 57,480 and 55,650 (A. fructiculosus agglutinin) and 59,600 and 56,380 (A. precatorius agglutinin). The proposed native molecular weights are 113,130 (. fructiculosus agglutinin) and 115,980 ( A. precatorius agglutinin), Alen treated with SDS and f - mercaptoethanol, the agglutinins were split into 3 bands each with corresponding agar molecular weights 38,460, 33,500 and 28,180 (,. fructiculosus agglutinin) and 40,790, 35,590 and 31,260 (A.precatorius agglutinin). The saline extracts from the two seeds did not interact with Afzelia africana polysaccharide in agar gel double diffusion studies. The toxicity of fructin and A. fructiculosus agglutinin was established on mice, with fructin being about 150 times more toxic than the agglutinin. Antisera formed against abrin and A. precatorius agglutinin did not interact with saline extracts of A. fructiculosus, fructin and A. fructiculosus agglutinin.
- ItemOpen AccessPurification and Physicochemical Characterization of Lectin from the Seeds of Treculia Africana Decne(2015-08-21) Adeniran, Olukemi AdetutuThe purification and characterization of the lectin from the seeds of Treculia africana Decne were carried out in order to determine some of its physicochemical properties as well as evaluate its toxicity in mice so as to understand the phenomenon of food intolerance caused by lectins. The protein in Treculia africana seeds was extracted by stirring the powdered seeds in phosphate buffered saline for 3 hours, kept overnight, and followed by centrifugation at 3000 rpm. The purification of the hemagglutinating protein was by ion-exchange chromatography on a DEAE-cellulose column followed by gel filtration on a Sephadex G-100 column. The apparent and subunit molecular weight were determined by gel filtration and SDS-polyacrylamide gel electrophoresis respectively. Detection of covalently bound carbohydrate was done by staining the gels after electrophoresis with periodic acid Schiff s reagent. The specificities of the crude extract and the purified protein were defined with human blood groups and sugars. The effects of temperature and pH on the hemagglutinating activity were determined by incubating aliquots of the protein at different temperature and pH values. The metal ions (Cu2+, Fe2+, Cr2+, Ni2+. Zn2+, Co2+, mg2+, Mn2+ and Ca2+) concentrations were determined by Atomic Absorption Spectroscopy. The effect of chelating agent (ethylenediaminetetra acetic acid EDTA) on the metal ions was investigated by dialyzing the protein against 10 mM EDTA and assaying for hemagglutination. Amino acid composition was analyzed with the Technicon sequential multi-sample amino acid analyzer. A 15-day acute toxicity of the lectin on mice was evaluated using standard procedures. Histopathological study was performed on some organs (brain, kidney, liver, lung, spleen and testis) of mice given intraperitoneal doses of the lectin. The results revealed that phosphate buffered saline extract of the seeds of Treculia africana agglutinated human red blood cells non-specifically. The hemagglutinating activity was inhibited by mannose with minimum inhibitory concentration of 0.8 mM and slightly enhanced by sorbose, dulcitol, glucose, and sorbitol. The purified lectin showed a single band in both denaturing and non-denaturing polyacrylamide gel electrophoresis. The subunit molecular weight as determined by SDS-PAGE and the native molecular weight as determined by gel filtration were 22,000 and 41,000 Daltons respectively. Amino acid composition analysis revealed that the protein contained 155 residues per subunit and was characterized by a high content of arginine, glutamic acid, aspartic acid, proline, cysteine, tyrosine and phenylalanine. Treatment of the protein with chelating agent (EDTA) had no inhibitory effect on the hemaglutinating activity. Analyses of metal ion contents revealed that the protein contained 42.13 mg/ml Cu2+, 3.30 mg/ml Fe3+, 21.01 mg/ml Mg2+, 9.24. mg/ml Mn2+ and 3.85 mg/ml Ca2+. The protein showed maximum activity over the pH range 3 – 7 and is relatively thermostable up to 50°C. Periodic acid Schiff's reagent staining showed that the protein was non-glycosylated. Although, the lectin was toxic with LD50 of 47.211 μg/g body weight of mice causing death instantaneously, there was no visible damaging effect on the organs of the mice following histopathological studies. In conclusion, the study revealed that seeds of Treculia Africana contained a lectin that was non-specific in its hemagglutinating property. The lectin exhibited properties and acute toxicity characteristic of ribosome-inactivating proteins (RIPS) with no damaging effect on the organs of the tested animals.
- ItemOpen AccessThe Role of Algae and Cyanobacteria in Arid Lands: a Review(1990) Isichei, Augustine O.Algae, cyanobacteria, and lichens occur in surface cryptogamic crusts, as free-living organisms in water bodies and within or on rocks in arid lands. The possible roles algae, cyanobacteria, and lichens could play in arid environments include physical improvement and protection of the soil, contribution of nitrogen to the arid ecosystem by nitrogen-fixing cyanobacteria and lichens, and primary biomass production for use as food and other secondary production. Physical improvement and protection of arid soils has potential in controlling desertification and rehabilitating arid lands. Culturing algae and cyanobacteria for biomass production, already being utilized in nonarid environments in agriculture, acquaculture, and now in the biochemical industry, has bright prospects in arid areas with their abundant sunshine. Primary production by the organisms can also be used for direct human and livestock consumption and in urban waste treatment. Biomass production can thus act as a means of resource diversification and therefore relieve pressure on fragile arid lands.
- ItemOpen AccessThe Role of Plant Resources in Nigeria's Economic Recovery Agenda(2005) Isichei, A. O.Basically, it is the performance of plants and chemical composition that we exploit for economic and cultural purposes. Our human world has been so closely tied to plants that it is difficult to imagine human existence without them. In all life on earth, plants are the only producers and all consumers are dependent upon plants for food, fibre, wood, energy and oxygen. Knowledge of plants, their habitats. structure, metabolism and inheritance is thus the basic foundation for human survival. Plants form the bedrock of life, being the first generator of oxygen in a reducing atmosphere that characterized the early earth. Plants are thus the roots of life and human material culture depends on them. The way a people incorporate plants into their cultural traditions, religions and even cosmologies reveals much about the people themselves. People rely on plants for much more than food and shelter and people use plants in so many ways that there are a few areas of human endeavour in which they do not play an important role. Plants have determined the course of human civilization - America was discovered during the course of the search of spices. Few societies can ignore the pivotal role of agriculture and forestry, both based essentially on plants. Several environmental crises such as global warming and biodiversity loss at their core, involve plants. It could indeed be that we are so closely linked that humans often take plants for granted, something to be left to the background and not worthy of serious economic consideration. But we met plants on our planet and they have defined our 'life zones'. The late appearance of humans on the evolutionary scene laid open to us a large variety of natural resources to exploit for food and plants were the natural choice, being the only organisms that had the capability to convert solar energy to chemical energy. From them we have learnt about life and it now looks as if we still have to depend on them to sort out our environmental crisis.
- ItemOpen AccessSynthesis and Characterization of Poly-8-Methylamino-Adenylic.(Obafemi Awolowo University, 1987) Elekwa, Iheanyichukwu; Falayan, J.O.A polynucleotide, poly-8-methylamino adenylic acid, was synthesized and hybridized with poly U. Adenosine-5-monophosphate purchased from BDN Chemical Corporation was brominated with bromine in Na-acetate buffer pH 3.9, stirred for 24 hours. The excess bromine was removed with some drops of concentrated sodium sulphite solution. It was then evaporated to dryness, on a rotatory evaporator at 37 oC and characterised. The product 8-Bromo-adenosine-5-Monphosphate, was methylaminated with methylamine in water, and refluxed for 48 hours at 65oC on an oil bath. Excess methylamine was removed with dilute sulphuric acid, while the product was evaporated to dryness and characterized. The synthesized methylamino adenosine-5-monophosphate was converted to its diphosphate analogue by the phophoro-morpholidate process. Orthophosphoric acid was used to introduce the phosphate group. The converted methylamino-adenosine-5-diphosphate was polymerized with the enzyme polynucleotide phophorylase PNPase, (EC 2.7.7.8) from Micrococcus luteus that was purchased from Boehringner Chemical Corporation. This enzyme PNPase is only specific for the diphosphate form. The polymerization was carried out in a reaction medium of MgCl2.6H2O EDTA (Ethylene diaminetetra-acetic acid) and tris buffer pH 9.0. It was incubated for 21 hours at 36oC, and characterized. The Poly-8-methyamino adenylic acid so synthesized was hybridized with poly U purchased from BDH- Chemical Corporation. The Job’s continuous variation method in KH2PO4 + K2HPO4 buffer pH 7.00 at 37oC was adopted. The polymer formed at 1:1 hybrid with Poly U. This satisfies some of the requirements for synthetic polynucleotide inducers. Some physico-chemical methods used in the characterization, included infra-red, ultra-violet, proton nuclear magnestic resonance and chromatographic methods. Complete UV spectra were recorded in the range of 200-400nm on Sp 8-400 (uv/vis) spectrophotometer. The infra-red spectra recorded using a sodium chloride cell in the range of 200-4000 cm-1 on Sp 3 -300 infra-red spectrophotometer. And, the Proton Nuclear Magnetic Resonance was recorded on Perkin Elmer Spectrophometer. The spots on the paper chromatography were detected and developed under UV light (at 254 nm wavelength).
- ItemOpen AccessTissue Culture Derived Plantlet Variation in Caladium humboldtii Schott(2007) Sakpere, A. M. A.; Adebona, A. C.Callus cultures were initiated from corm and petiole explants of C. humboldtii on Murashige and Skoog's basal medium (MS) supplemented with 2,4-Dichlorophenoxyacetic acid (2, 4-D) (0.4mg/l - 1.6mg/l) in combination with Kinetin (1mg/l) in the dark. Callus was induced on media supplemented with 0.8mg/l 2,4-Dichlorophenoxyacetic acid (2, 4-D) in combination with kinetin (1mg/l) and callus induced on this media showed the best growth. Direct regeneration potential was higher in corm than in leaf explants. Regeneration was not achieved in petiole explants. De novo plant regeneration from callus cultures was not achieved and somatic embryogenesis did not yield any plantlets. Morphological differences were observed among the regenerated plantlets of C. humboldtii on Murashige and Skoog medium (MS) supplemented with 2, 4-D (0.4mg/l) in combination with 1mg/l Kinetin. Polyacrylamide gel electrophoresis showed only 1 band each in the control and in the regenerants, however, the position of the bands were different. The result indicates that variation has occurred during in vitro culture. In conclusion, it has not been possible to generate plantlets from callus and it has also not been possible to advance the callus beyond the early stage of embryo development. The findings however include production of a new cultivar of C. humboldtii, initiation/growth of callus and direct regeneration of plantlets in the dark.