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Research Detail

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Dilruba Yeasmin
Department of Botany, University of Rajshahi, Rajshahi 6205, Bangladesh

Rawnak Jahan Swarna
Department of Botany, University of Rajshahi, Rajshahi 6205, Bangladesh

Mst. Samima Nasrin
Department of Botany, University of Rajshahi, Rajshahi 6205, Bangladesh

,Sarwar Parvez
Department of Botany, University of Rajshahi, Rajshahi 6205, Bangladesh

Mohammad Firoz Alam
Department of Botany, University of Rajshahi, Rajshahi 6205, Bangladesh

Chrysanthemum morifolium Ramat. is an important medicinal plant. To learn more about properties of this plant, the present study was aimed to evaluate the phytochemical analysis and antioxidant activity of three colours (pink, yellow and white) flower of Chrysanthemum morifolium. Spot phytochemical screening of these three colours of C. morifolium in the ethanol extract showed that alkaloids, phenols, flavonoids, glycoside and terpenoids were present in studied three colours (pink, white and yellow) flower but saponin and tannin were absent in pink and yellow flower. Free radical-induced oxidative stress is the root cause for many human disease. Naturally occurring antioxidant supplements from plants are vital to counter the oxidative damage in cells. An antioxidant activity of these three flower colours (pink, yellow and white) Chrysanthemum morifolium were examined through DPPH antioxidant assay. The sample showed significant antioxidant activity. Where IC50 value of the three flower extracts were 10.00mg/ml, 11.00mg/ml and 40.00mg/ml for white, pink and yellow flower extracts respectively. In ascorbic acid the IC50 value was calculated 11.50 mg/ml. The phytochemical analysis supports antioxidant properties of these flower colours. So, for comparing among pink, white, yellow flower, white flower of chrysanthemum was found good for potential phytochemical and antioxidant properties

  Chrysanthemum, Phytochemical analysis, Antioxidant, DPPH, Free radicals.
  Department of botany, Rajshahi University Rajshahi-6205, Bangladesh,
  
  
  Crop-Soil-Water Management
  Flower

In this work, ethanol extracts of three colours (pink, yellow and white) flower of Chrysanthemum morifolium were examined for their secondary metabolites content and antioxidant activities.

Plant material- White and yellow colour flower of chrysanthemum morifolium were collected from local farmer of Jessore, Bangladesh and pink colour flower of chrysanthemum morifolium was collected from local farmer of Rajshahi, Bangladesh. The   plant   material   was   collected   in   December- January,  2014.  Dr.  A.  H.   M.  Mahbubur  Rahman, Associate  Professor,  Department  of  botany,  Rajshahi University Rajshahi-6205, Bangladesh, confirmed the taxonomic identification of the plant. Chemicals and Reagents-2, 2-Diphenyl-1-picrylhydrazyl (DPPH), ascorbic acid, methanol,  ethanol,  Dragendroff’s,  Hager’s,  Mayer’s, Wagner’s and Tannic acid reagents. Spot phytochemical analysis Preparation of sample- Initially well washed flowers were dried in hot air oven. The dried materials were coarsely powdered as a fine powder. Spot phytochemical screening of three colours (pink, yellow and white) flower of C. morifolium were carried out by using the following protocols as described below for the presence of alkaloids, flavonoids, glycosides, saponins, tannins, terpenoids and phenols. Determination of Alkaloids- 5 g fine powder was mixed up to moistered with 10 ml 2%  HCl  and  heated  in  water  at  60 °C  for  one  hour. After    cooling    the    sample    was    filtered    through Whatmann  No.  1  filter  paper.  Two  drops  of  filtrates were put on a microscopic groove slide with one drop of    the    alkaloid    detecting    reagent.    The    relative abundance of precipitate, if any, formed in the plant sample   with   the   reagents   was   considered   as   the presence of alkaloid (Aplin and Cannon 1971).  Determination of Flavonoids- About  10  g  plant  sample  was  extracted  with  20  ml ethanol  (1:2)  in  aspirator  bottle  by  soaking  about  72 hours. After that  few  drops of  conc. HCl were added to  the  alcoholic  extract  resulting  red  color,  indicates the presence of flavonoids (Farnsworth 1985).  Determination of Glycosides- A  small  amount  of  sample  solution  was  mixed  with 2ml of  glacial acetic acid containing 1-2 drops  of 2% solution of FeCl3. The mixture was then poured into another   test   tube   containing   2ml   of   concentrated H2SO4.  A  brown  ring  at  the  interphase  indicated  the presence   of   cardiac   glycosides   (Trease   and   Evans 1989). Determination of Saponins- 20  ml  water  is  added  to  150  mg  fine  powder  and shaken vigorously;  layer of foam formation  indicates the presence of saponins (Siddiqui and Ali 1997). Determination of Tannins- 2g  fine  powder  was  extracted  with  10  ml  distilled water   (1:5),   and   was   boiled   for   about   20   to   25 minutes.  After  cooling  the  extract  was  filtered.  The filtrate was taken on 3 microscopic slides, two drops on each.  Then to the first slide one drop 10% NaCl, to the  second  1%  gelatin  and  to  the  third  1%  gelatin  + 10%  NaCl  were  added.  The  appearance  of  a  white precipitate  on  the  second  and  third  was  taken  as positive test for tannins (Wall et al.1954).  Determination of Terpenoids- 2ml  of  sample  was  mixed  in  5ml  of  chloroform  and concentrated H2SO4  2ml was carefully added to form layer. A reddish brown coloration of the interface was formed show positive   result   for   the   presence   of terpenoids (Harborne 1973). ?Determination of Phenols- 5ml of sample was mixed with 2ml of 2% solution of FeCl3. A blue-green or black coloration indicated the presence of phenols.  Antioxidant activity- Antioxidant activity of three colours (pink, yellow and white)  flower  of  C.  morifolium  were  estimated  for their  free  radical  scavenging  activity  by  using  DPPH (2, 2-Diphenyl-1-Picrylhydrazyl) as described by Hsu et al. (2007) with some modification.  Experimental procedure of Antioxidant activity test- First, various concentrations like 20, 40, 60, 80, 100 mg/ml of sample in methanol were prepared. 2 ml of methanol  solution  of  plant  sample  or  standard  at different concentrations  was taken in test tube.  3 ml of 0.1 mm methanol solution of DPPH was added into the test tube.  The test tube was incubating at room temperature for 30 minutes in dark place to complete the reaction. Then the absorbance of the solution was measured at 517  nm  using  a  spectrophotometer  against  control. Ascorbic    acid    was    used    as    standards    (positive control).  Then  the  percentage  (%)  inhibition  activity was calculated according to Pavlov et al. (2002).  % I= {(AO– A1)/AO}*100; Where, AO  is the absorbance of the control, and A1  is the  absorbance  of  the  sample  or  standard.  Sample was  analyzed  in  two  replications  and  data  presented as  mean  (±)  standard  deviation  (SD).  Then  %  of inhibition  was  plotted  against  blank  concentration and  from  the  graph  IC50  was  calculated.  IC50   value, the    concentration    of    sample    required    for    50% scavenging   of   DPPH   free   radical   are   completed (Mandal et al., 2009). Statistical analysis- Statistical analysis (ANOVA) and Least Significant Difference (LSD) test was used to speculate further if there was a significant difference within varieties, various concentrations. P values <0.05 were considered as significant.

  International Journal of Biosciences | IJB |, Vol. 9, No. 2, p. 69-77, 2016
  http://dx.doi.org/10.12692/ijb/9.2.69-77
Funding Source:
1.   Budget:  
  

From the above discussion, it can be concluded that as chrysanthemum flower can be used to cure some common and other various diseases. Qualitative phytochemical screening and nutraceutical like antioxidant activity of chrysanthemum suggests that we can use chrysanthemum products as herbal medicine and with the help of the indigenous knowledge. We can avoid production and import of many synthetic medicines and also can boost our economy by exporting our products because the current inorganic drugs in the market have several side effects and an effective means to sustain is still a challenge.

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