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Node culture of Bacopa MoNNieri
aNd
phytocheMical assessMeNt of regeNerate
INSTITUTE OF GENETIC ENGINEERING
NAME-PAYEL GHOSH
M.Sc BIOTECHNOLOGY
Specialization โ€“Agricultural Biotechnology
ROLL-21016012013
: DR.MADHUMITA.J.MUKHOPADHYAY
Supervised by
INTRODUCTIONINTRODUCTION
What isWhat is
MicropropagatioNMicropropagatioNThe aseptic method of clonal propagation that is
carried out on a miniature scale under aseptic
conditions.
The advantage is that in a
relatively short time and space
a large number of plants are
obtained.
The advantage is that in a
relatively short time and space
a large number of plants are
obtained.
๏ถ type of MicropropagatioNtype of MicropropagatioN
1.Direct micropropagation
2.Indirect micropropagation
๏ถ type of MicropropagatioNtype of MicropropagatioN
1.Direct micropropagation
2.Indirect micropropagation
Advantages of micropropagationAdvantages of micropropagation
๏ƒ˜ From one to many propagules rapidly
๏ƒ˜ Multiplication in controlled lab conditions
๏ƒ˜ Continuous propagation year round
๏ƒ˜ Potential for disease-free propagules
๏ƒ˜ Inexpensive per plant once established
๏ƒ˜ Precise crop production scheduling
๏ƒ˜ Reduce stock plant space
๏ƒ˜ Long-term germplasm storage
๏ƒ˜ Production of difficult-to-propagate species
DisadvantagesDisadvantagesDisadvantagesDisadvantages
๏ƒ˜ Specialized equipment/facilities required
๏ƒ˜ More technical expertise required
๏ƒ˜ Protocols not optimized for all species
๏ƒ˜ Plants produced may not fit industry standards
๏ƒ˜ Relatively expensive to set up
Steps of MicropropagationSteps of Micropropagation
Micropropagation involved in 5 steps:
aBout
Bacopa
Taxonomic positionTaxonomic position
Kingdom:- Plantae
Division- Angiosperms
Class- Eudicots
Order- Lamiales
Family- scrophulariaceae
Genus- Bacopa
Species-
B.monnieri
HabitHabit Terrestrial ,Annual, procumbent, herb,
StemStem herbaceous, branched, solid with prominent nodes
and internodes, cylindrical, green in colour.
RootRoot tap and adventious root
Leaf:Leaf: opposite decussate, sessile, estipulate simple
FlowerFlower Pedicillate, Ebracteates, bracteolate complete,
bisexual, zygomorphic, hypogunos, cyclic
diclamydiouus, erect, size-1cm*1cm; odorless;
CalyxCalyx gamosepalous, inferior, persistant, irregular ,
CorollaCorolla Gamopetalous, deciduous, infiriour, irregular,
campanulate,color-white with tinger purple
AndrociumAndrocium stamen-4, epipetalous, antisepalous,
infiriour.didynomous, anther bilocular, black,
dorsifixed
GynociumGynocium syncarpous,carpels-2ovary superior,ovoidin shape
style -1stigma-2
Fruit:Fruit: Capsule
characteristic of
Bacopa
uses of Bacopa
MediciNal useMediciNal use
โ€ขBacopa is a great neurotonic, immuno-
modulator, adaptogen, tranquilizing,
memory and learning enhancing,
cerebral activator, anti-ulcer,
antispasmodic, antiasthmatic ayurvedic
herb.
โ€ขAlso used as herbal supplement in
Epilepsy, anxiety and depression.
โ€ขIt is also hlep to cure the liver cancer.
๏ถMainly used as vegetable
๏ถextract also used as medicine , food
industry (as jam )
๏ถIt is also used in cosmetic industry as dust .
Leaf exactract used to make oil
๏ถIt is also used in ornamentation
Develop a rapid mass propagation protocol of Bacopa monnieri.
Standardization of growth regulator for shooting
and rooting in order to achieve quality plantlet.
Phytochemical screening of Bacopa monnieri
Why Bacopa monnieri
Bacopa have a wide variety of uses specially used as traditional
medicine
The medicine is important to presence for alkaloid (Bacoside โ€“A
Bacoside โ€“B)
Due to over exploitation Bacopa is already under threatened plant
list.
As an Ex situ conservation method in vitro micropropagation is
necessary for Bacopa sp.
Bacoside โ€“B Bacoside โ€“A
Glycosides of 20-deoxy derivatives of jujubogenin and
pseudojujubogenin from Bacopa monnieri. ,
Planta Med. 2011 ;73(4):380-3.
A detailed phytochemical investigation of an extract of Bacopa monnieri resulted in the
isolation of two new glycosides . They have been identified as glycosides of the 20-deoxy
derivatives of jujubogenin and pseudojujubogenin. The structures were established by
different spectroscopic methods that included 1D and 2D NMR experiments. The
compounds when tested exhibited mild to moderate cytotoxicity towards non-
cancerous kidney cell lines
Neuroprotective role of Bacopa monnieri extract in epilepsy and effect of
glucose supplementation during hypoxia: glutamate receptor gene expression.
G. Phani Kumar and Farhath Khanum, Pharmacognosy Rev. (2012) 6(12) 81-90.
neuroprotective role of Bacopa monnieri extract in epilepsy was found.
New functional leads for Alzheimer's disease has been provided for Bacopa sp.
Ayurvedic medicinal plants for Alzheimer's disease: a review
Rammohan V Rao, Olivier Descamps, [., and Dale E Bredesen
Alzheimer's Res. Ther. (2012) 4(3):22
Tissue Culture, Phytochemical & Pharmacological Study of Bacopa
Monnieri
Arun Sundriyal1, Devinder Singh Rawat2 & Amit Kumar Singh
Asian Journal of Biochemical and Pharmaceutical Research Issue 1(Vol. 3) 2013, 243-260
Establishment of axillary bud, organogenetic plant and callus culture through different plant growth
regulator has been reporteds. Multiplication and maintenance of cultures are also mentioned
๏ƒ˜
Nodes of Bacopa monnieri
๏ƒ˜
TWEEN 20 (5% v/v)[liquid detergent]
๏ƒ˜
BAVISTINE(0.1%)
๏ƒ˜
Chlorochol-d
๏ƒ˜
HgCl2
๏ƒ˜
MS MEDIUM (Murashige & Skoogโ€™s)
๏ƒ˜
SUCROSE(3% & 6%)
๏ƒ˜
NICOTINIC ACID(0.5mg/l)
๏ƒ˜
PYRIDOXINE HCL
๏ƒ˜
GLUTAMINE WITH DIFFERENT GROWTH REGULATORS
๏ƒ˜
COOL WHITE FLUORESECENT TUBES
๏ƒ˜
BAP WITH NAA(DIFFERENT CONCENTRATION)
โ€ข
SUGAR = 30 mg
โ€ข
Sulphate = 10 ml
โ€ข
Phosphate = 10 ml
โ€ข
Hallide = 10 ml
โ€ข
Nitrate = 20 ml
โ€ข
FeEDTA = 10 ml
โ€ข
Glycine = 2 ml
โ€ข
Nicotinic acid =500 ยตl
โ€ข
Pyridoxin = 500 ยตl
โ€ข
Thymine HCl = 100 ยตl
โ€ข
Inositol = 100 mg
โ€ข
Adenine sulphate = 100 mg
Volume make up to 1000 ml by distiled water
โ€ข
Ager = 8gm
โ€ข
Growth regulator are added
PREPERATION OF MS MEDIUM (1000 ml) for MICROPROPAGATIONPREPERATION OF MS MEDIUM (1000 ml) for MICROPROPAGATION
1 .STERILIZATION
-Glasswares washed in hot water.
-Kept in chromic acid overnight.
-Next day jars were kept in soap water overnight.
-Cleaned with dist.water.
-Kept in Hot Air Oven.
2. PREPARATION OF
MEDIA
In a measuring cylinder, all
the components of required quantity
were taken from the stock solutions.
The final volume was made up with
double distilled water.
The requisite quantities of growth
regulators were solutions.
The pH was adjusted to 5.6 using either
1N NaOH or 1N HCl
๏‚ง
The media were then poured
into culture bottles, plugged
and wrapped with brown
paper.
๏‚ง
The tubes containing media
were then autoclaved.
๏‚ง
Agar (0.8%) was added
to the medium and
dissolved by boiling.
MS + 1 mg/l BAP
+ 1 mg/l NAA
MM2(Multiplicati
on Media)
MS + 2 mg/l BAP
+ 1mg/l NAA
IM1
MS + 1 mg/l BAP
+ 0.5 mg/l NAA
IM(Induction
Media)
MS basal as
control
MS
Composition of mediausing different concentration of
BAPand NAA for shoot bud multiplication
Also few other concentrations of NAA and BAP were used
Tween
20
โ€ขNodes from healthy mother plant(explant) of Bacopa
monnieri
โ€ขWashed thoroughly under tap water for 5
mins
โ€ขWashed thoroughly under tap water for 5
mins
โ€ขTreated with tween-20,bavistin, chlorocol d
separately and washed by tap water and distill
water
โ€ขThis treatment is done 3 times
MethodMethod
CONTINUEDโ€ฆ
Then transferred to MS medium[with BAP/NAA]
Axillary bud break was achieved in 2 weeks in all aseptic cultures
on MS medium supplemented with 0.5-4.0 mg/l BAP
After 5 week of subculture duration it was noticed that the best in vitro
shoot multiplication with sizeable shoots was obtained
The shoot was transferred to half MS Basal media with IBA for
rooting
The rooted shoot formed lets ready for field transfer
subculturing of all cultures at every week on the same
medium
Composition of media using different concentration of
auxin and cytokinin for shoot bud multiplication
Auxilary Bud Induction (10 days) in MS1 Medium
MS1=MS basal + 0.1 mg/l BAP + 0.1 mg/l NAA
Auxilary Bud Induction (10 days) in MS2 Medium
MS2MS2== MS basal media+MS basal media+
0.5mg/l BAP+0.1mg/l NAA
MS2MS2== MS basal media+MS basal media+
0.5mg/l BAP+0.1mg/l NAA
Auxilary Bud Induction (10 days) in MS3
Medium
MS 3= MS media+1mg/l BAP + 0.1MS 3= MS media+1mg/l BAP + 0.1
mg/l NAAmg/l NAA
Multiple Shoot Proliferation in
MS(3)Medium
MS3= MS basal media+
1mg/l BAP+ 0.1 mg/l NAA
Multiple Shoot Proliferation in
MS(4) Medium
MS 4= MS basal media+ 4mg/l BAP
+0.1 mg NAA
Multiple Shoot Proliferation in
MS(5) Medium
B1N1
MS 5=MS basal Media
1mg/l BAP +1mg/l NAA
Graphical representation of length of
shoots in different medium
THE BEST RESULT FOR MS5 MEDIA
THAT CONTAIN BAP 1mg/l & NAA
1mg/l as GROWTH REGULATORS.โ€ฆ.
THE BEST RESULT FOR MS5 MEDIA
THAT CONTAIN BAP 1mg/l & NAA
1mg/l as GROWTH REGULATORS.โ€ฆ.
IN VITRO RESPONSES OF THE MEDIUM ONIN VITRO RESPONSES OF THE MEDIUM ON
INDUCTION OF ROOTS OFINDUCTION OF ROOTS OF Bacopa monnieriBacopa monnieri
Conc. Of IBA
(mg/l)
Average no. of
roots
Root length (cm)
0.2 1.81ยฑ0.62 2.11ยฑ0.85
0.4 2.63ยฑ0.62 3.00ยฑ1.2
0.6 4.12ยฑ0.62 4.50ยฑ0.96
0.8 5.01ยฑ0.62 5.23ยฑ0.89
1.0 5.81ยฑ0.62 6.99ยฑ0.92
Graphical representation of length of
root in different conc. Of IBA
no
Of
Root
PHYTOCHEMICAL SCERRENING
OF BACOPA
Bacopa leaves are collected and wash thoroughly by tap water
Crushed them in 2 part
Ethanol extract solution Aqua's solution
Preparation of sample solution from regenerated plantPreparation of sample solution from regenerated plant
Solution heated on for 20mins in
water bath
N.B. : Following test are done by this solution
Solution heated on for 5 mins in
water bath
Half of them absorved by alcohol and other s absorbed by water for 24 hrs.
Test of Market sample Culture sample observation conclusion
Eth solution Aq solution Eth solution Aq solution
pholobatannin
s
Sample+
1%HCl
Sample+
1%HCl
Red ppt are
found
pholobatanni
ns
Present
Flavonoid Sample+conc.H
2SO4+5ml
NH4OH
Sample+conc.H
2SO4+5ml
NH4OH
Yellow color
appeared
Flavonoid
Are present
Steroid 2 ml Acetic
anhydride+0.5
ml sample+2ml
H2SO4
2 ml Acetic
anhydride+0.5
ml sample+2ml
H2SO4
Violet blue
green color
appeared
Steroid are
present
Terpinods Sample+2mlCH
3Cl+conc.H2SO4
Sample+2ml
CH3Cl+conc.H2S
O4
Radish brown
color
Terpinodes
are present
Cardiac
glycoside
2ml glacial
acetic acid
+ferric chloride
solution+extrac
t+conc H2SO4
2ml glacial
acetic acid
+ferric chloride
solution+extrac
t+conc H2SO4
Brown ring
formation
Cardiac
glycoside
are present
Amino acid Sample +few
drops
ninhydrin+wat
er bath heating
Sample +few
drops
ninhydrin+wat
er bath heating
Violet color Amino acid
are present
Test of pholobatannins:
Sample solution +1%HCl=
๏‚ง Red ppt are found
Pholobatannins test Flavonoid test
Test of flavonoid
Sample+conc.H2SO4+
5ml NH4OH =
Yellow color appeared
โ€ข Test of Steroid
2 ml Acetic anhydride+0.5ml
ethanolic sample solution+2ml
H2SO4 =Violet blue green color
appeared and ring formation
โ€ข Test of Terpinoid
โ€ข Sample+2mlCH3Cl+conc.
H2SO4 = Radish brown
color
โ€ข Test of cardiac glycoside
โ€ข 2ml glacial acetic acid
+ferric chloride
solution+extract+conc
H2SO4 = yellow color
appeared
โ€ข Test of amino acid
โ€ข Sample +few drops
ninhydrin+water bath
heating = Violet color
appeared
1.0 mg/l of BAP &1.0mg/l of NAA gave the best result for in
vitro shoot formation.
The study showed addition of 1mg/l IBA gave profuse of rooting.
The similarity in the Phytochemichal analysis in both
regenerated and control one for pholobatannins, cardiac
glycoside, Steroid , Terpinoid and amino acid showed a
possibility of using these regenerated plants for other uses.
A quick and easy micropropagation protocol of the medicinal
plant Bacopa monnieri has been established
ConClusion
โ€ข Glycosides of 20-deoxy derivatives of jujubogenin and pseudojujubogenin from Bacopa
monniera. , Planta Med. 2011 ;73(4):380-3.
Neuroprotective role of Bacopa monnieri extract in epilepsy and effect of glucose
supplementation during hypoxia: glutamate receptor gene expression.G. Phani Kumar and
Farhath Khanum, Pharmacognosy Rev. (2012) 6(12) 81-90.
Ayurvedic medicinal plants for Alzheimer's disease: a review Rammohan V Rao, Olivier
Descamps, [., and Dale E Bredesen Alzheimer's Res. Ther. (2012) 4(3):22
Singh RH, Narsimhamurthy K, Singh G
Neuronutrient impact of Ayurvedic Rasayana therapy in brain aging. Biogerontology. 2008
Dec;9(6):369-74. doi: 10.1007/s10522-008-9185-z.
Kulhari A1, Sheorayan A1, Bajar S2, Sarkar S3, Chaudhury A1, Kalia RK1.
Investigation of heavy metals in frequently utilized medicinal plants collected from
Springerplus. 2013 Dec 17;2:676. doi: 10.1186/2193-1801-2-676.
Srivastava P, Raut HN, Puntambekar HM, Desai AC.
Stability studies of crude plant material of Bacopa monnieri and quantitative deter
Phytochem Anal. 2012 Sep-Oct; 23(5):502-7. Doi: 10.1002/pca.234
Williams R, Mรผnch G, Gyengesi E, Bennett L.
Bacopamonnieri (L.) exerts anti-inflammatory effects on cells of the innate immune
Food Funct. 2014 Jan 22.
I AM MOST THANKFUL TO
PROF.A.CHAKRAVARTHY
DR.SUDIPA CHAKRAVARTHY
DR.MADHUMITA.J.MUKHOPADHYA
AND
DEBRAJ SIR
FOR HELPING ME WITH THIS PROJECT.
bramhi the medicinal plant

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bramhi the medicinal plant

  • 1. Node culture of Bacopa MoNNieri aNd phytocheMical assessMeNt of regeNerate INSTITUTE OF GENETIC ENGINEERING NAME-PAYEL GHOSH M.Sc BIOTECHNOLOGY Specialization โ€“Agricultural Biotechnology ROLL-21016012013 : DR.MADHUMITA.J.MUKHOPADHYAY Supervised by
  • 3. What isWhat is MicropropagatioNMicropropagatioNThe aseptic method of clonal propagation that is carried out on a miniature scale under aseptic conditions. The advantage is that in a relatively short time and space a large number of plants are obtained. The advantage is that in a relatively short time and space a large number of plants are obtained. ๏ถ type of MicropropagatioNtype of MicropropagatioN 1.Direct micropropagation 2.Indirect micropropagation ๏ถ type of MicropropagatioNtype of MicropropagatioN 1.Direct micropropagation 2.Indirect micropropagation
  • 4. Advantages of micropropagationAdvantages of micropropagation ๏ƒ˜ From one to many propagules rapidly ๏ƒ˜ Multiplication in controlled lab conditions ๏ƒ˜ Continuous propagation year round ๏ƒ˜ Potential for disease-free propagules ๏ƒ˜ Inexpensive per plant once established ๏ƒ˜ Precise crop production scheduling ๏ƒ˜ Reduce stock plant space ๏ƒ˜ Long-term germplasm storage ๏ƒ˜ Production of difficult-to-propagate species DisadvantagesDisadvantagesDisadvantagesDisadvantages ๏ƒ˜ Specialized equipment/facilities required ๏ƒ˜ More technical expertise required ๏ƒ˜ Protocols not optimized for all species ๏ƒ˜ Plants produced may not fit industry standards ๏ƒ˜ Relatively expensive to set up
  • 5. Steps of MicropropagationSteps of Micropropagation
  • 8. Taxonomic positionTaxonomic position Kingdom:- Plantae Division- Angiosperms Class- Eudicots Order- Lamiales Family- scrophulariaceae Genus- Bacopa Species- B.monnieri
  • 9. HabitHabit Terrestrial ,Annual, procumbent, herb, StemStem herbaceous, branched, solid with prominent nodes and internodes, cylindrical, green in colour. RootRoot tap and adventious root Leaf:Leaf: opposite decussate, sessile, estipulate simple FlowerFlower Pedicillate, Ebracteates, bracteolate complete, bisexual, zygomorphic, hypogunos, cyclic diclamydiouus, erect, size-1cm*1cm; odorless; CalyxCalyx gamosepalous, inferior, persistant, irregular , CorollaCorolla Gamopetalous, deciduous, infiriour, irregular, campanulate,color-white with tinger purple AndrociumAndrocium stamen-4, epipetalous, antisepalous, infiriour.didynomous, anther bilocular, black, dorsifixed GynociumGynocium syncarpous,carpels-2ovary superior,ovoidin shape style -1stigma-2 Fruit:Fruit: Capsule characteristic of Bacopa
  • 10. uses of Bacopa MediciNal useMediciNal use โ€ขBacopa is a great neurotonic, immuno- modulator, adaptogen, tranquilizing, memory and learning enhancing, cerebral activator, anti-ulcer, antispasmodic, antiasthmatic ayurvedic herb. โ€ขAlso used as herbal supplement in Epilepsy, anxiety and depression. โ€ขIt is also hlep to cure the liver cancer.
  • 11. ๏ถMainly used as vegetable ๏ถextract also used as medicine , food industry (as jam ) ๏ถIt is also used in cosmetic industry as dust . Leaf exactract used to make oil ๏ถIt is also used in ornamentation
  • 12.
  • 13. Develop a rapid mass propagation protocol of Bacopa monnieri. Standardization of growth regulator for shooting and rooting in order to achieve quality plantlet. Phytochemical screening of Bacopa monnieri
  • 14. Why Bacopa monnieri Bacopa have a wide variety of uses specially used as traditional medicine The medicine is important to presence for alkaloid (Bacoside โ€“A Bacoside โ€“B) Due to over exploitation Bacopa is already under threatened plant list. As an Ex situ conservation method in vitro micropropagation is necessary for Bacopa sp. Bacoside โ€“B Bacoside โ€“A
  • 15.
  • 16. Glycosides of 20-deoxy derivatives of jujubogenin and pseudojujubogenin from Bacopa monnieri. , Planta Med. 2011 ;73(4):380-3. A detailed phytochemical investigation of an extract of Bacopa monnieri resulted in the isolation of two new glycosides . They have been identified as glycosides of the 20-deoxy derivatives of jujubogenin and pseudojujubogenin. The structures were established by different spectroscopic methods that included 1D and 2D NMR experiments. The compounds when tested exhibited mild to moderate cytotoxicity towards non- cancerous kidney cell lines Neuroprotective role of Bacopa monnieri extract in epilepsy and effect of glucose supplementation during hypoxia: glutamate receptor gene expression. G. Phani Kumar and Farhath Khanum, Pharmacognosy Rev. (2012) 6(12) 81-90. neuroprotective role of Bacopa monnieri extract in epilepsy was found.
  • 17. New functional leads for Alzheimer's disease has been provided for Bacopa sp. Ayurvedic medicinal plants for Alzheimer's disease: a review Rammohan V Rao, Olivier Descamps, [., and Dale E Bredesen Alzheimer's Res. Ther. (2012) 4(3):22 Tissue Culture, Phytochemical & Pharmacological Study of Bacopa Monnieri Arun Sundriyal1, Devinder Singh Rawat2 & Amit Kumar Singh Asian Journal of Biochemical and Pharmaceutical Research Issue 1(Vol. 3) 2013, 243-260 Establishment of axillary bud, organogenetic plant and callus culture through different plant growth regulator has been reporteds. Multiplication and maintenance of cultures are also mentioned
  • 18.
  • 19. ๏ƒ˜ Nodes of Bacopa monnieri ๏ƒ˜ TWEEN 20 (5% v/v)[liquid detergent] ๏ƒ˜ BAVISTINE(0.1%) ๏ƒ˜ Chlorochol-d ๏ƒ˜ HgCl2 ๏ƒ˜ MS MEDIUM (Murashige & Skoogโ€™s) ๏ƒ˜ SUCROSE(3% & 6%) ๏ƒ˜ NICOTINIC ACID(0.5mg/l) ๏ƒ˜ PYRIDOXINE HCL ๏ƒ˜ GLUTAMINE WITH DIFFERENT GROWTH REGULATORS ๏ƒ˜ COOL WHITE FLUORESECENT TUBES ๏ƒ˜ BAP WITH NAA(DIFFERENT CONCENTRATION)
  • 20.
  • 21.
  • 22. โ€ข SUGAR = 30 mg โ€ข Sulphate = 10 ml โ€ข Phosphate = 10 ml โ€ข Hallide = 10 ml โ€ข Nitrate = 20 ml โ€ข FeEDTA = 10 ml โ€ข Glycine = 2 ml โ€ข Nicotinic acid =500 ยตl โ€ข Pyridoxin = 500 ยตl โ€ข Thymine HCl = 100 ยตl โ€ข Inositol = 100 mg โ€ข Adenine sulphate = 100 mg Volume make up to 1000 ml by distiled water โ€ข Ager = 8gm โ€ข Growth regulator are added PREPERATION OF MS MEDIUM (1000 ml) for MICROPROPAGATIONPREPERATION OF MS MEDIUM (1000 ml) for MICROPROPAGATION
  • 23. 1 .STERILIZATION -Glasswares washed in hot water. -Kept in chromic acid overnight. -Next day jars were kept in soap water overnight. -Cleaned with dist.water. -Kept in Hot Air Oven. 2. PREPARATION OF MEDIA In a measuring cylinder, all the components of required quantity were taken from the stock solutions. The final volume was made up with double distilled water. The requisite quantities of growth regulators were solutions. The pH was adjusted to 5.6 using either 1N NaOH or 1N HCl ๏‚ง The media were then poured into culture bottles, plugged and wrapped with brown paper. ๏‚ง The tubes containing media were then autoclaved. ๏‚ง Agar (0.8%) was added to the medium and dissolved by boiling.
  • 24. MS + 1 mg/l BAP + 1 mg/l NAA MM2(Multiplicati on Media) MS + 2 mg/l BAP + 1mg/l NAA IM1 MS + 1 mg/l BAP + 0.5 mg/l NAA IM(Induction Media) MS basal as control MS Composition of mediausing different concentration of BAPand NAA for shoot bud multiplication Also few other concentrations of NAA and BAP were used
  • 25. Tween 20 โ€ขNodes from healthy mother plant(explant) of Bacopa monnieri โ€ขWashed thoroughly under tap water for 5 mins โ€ขWashed thoroughly under tap water for 5 mins โ€ขTreated with tween-20,bavistin, chlorocol d separately and washed by tap water and distill water โ€ขThis treatment is done 3 times MethodMethod CONTINUEDโ€ฆ
  • 26. Then transferred to MS medium[with BAP/NAA] Axillary bud break was achieved in 2 weeks in all aseptic cultures on MS medium supplemented with 0.5-4.0 mg/l BAP After 5 week of subculture duration it was noticed that the best in vitro shoot multiplication with sizeable shoots was obtained The shoot was transferred to half MS Basal media with IBA for rooting The rooted shoot formed lets ready for field transfer subculturing of all cultures at every week on the same medium
  • 27.
  • 28. Composition of media using different concentration of auxin and cytokinin for shoot bud multiplication
  • 29. Auxilary Bud Induction (10 days) in MS1 Medium MS1=MS basal + 0.1 mg/l BAP + 0.1 mg/l NAA
  • 30. Auxilary Bud Induction (10 days) in MS2 Medium MS2MS2== MS basal media+MS basal media+ 0.5mg/l BAP+0.1mg/l NAA MS2MS2== MS basal media+MS basal media+ 0.5mg/l BAP+0.1mg/l NAA
  • 31. Auxilary Bud Induction (10 days) in MS3 Medium MS 3= MS media+1mg/l BAP + 0.1MS 3= MS media+1mg/l BAP + 0.1 mg/l NAAmg/l NAA
  • 32. Multiple Shoot Proliferation in MS(3)Medium MS3= MS basal media+ 1mg/l BAP+ 0.1 mg/l NAA
  • 33. Multiple Shoot Proliferation in MS(4) Medium MS 4= MS basal media+ 4mg/l BAP +0.1 mg NAA
  • 34. Multiple Shoot Proliferation in MS(5) Medium B1N1 MS 5=MS basal Media 1mg/l BAP +1mg/l NAA
  • 35. Graphical representation of length of shoots in different medium THE BEST RESULT FOR MS5 MEDIA THAT CONTAIN BAP 1mg/l & NAA 1mg/l as GROWTH REGULATORS.โ€ฆ. THE BEST RESULT FOR MS5 MEDIA THAT CONTAIN BAP 1mg/l & NAA 1mg/l as GROWTH REGULATORS.โ€ฆ.
  • 36. IN VITRO RESPONSES OF THE MEDIUM ONIN VITRO RESPONSES OF THE MEDIUM ON INDUCTION OF ROOTS OFINDUCTION OF ROOTS OF Bacopa monnieriBacopa monnieri Conc. Of IBA (mg/l) Average no. of roots Root length (cm) 0.2 1.81ยฑ0.62 2.11ยฑ0.85 0.4 2.63ยฑ0.62 3.00ยฑ1.2 0.6 4.12ยฑ0.62 4.50ยฑ0.96 0.8 5.01ยฑ0.62 5.23ยฑ0.89 1.0 5.81ยฑ0.62 6.99ยฑ0.92
  • 37. Graphical representation of length of root in different conc. Of IBA no Of Root
  • 39. Bacopa leaves are collected and wash thoroughly by tap water Crushed them in 2 part Ethanol extract solution Aqua's solution Preparation of sample solution from regenerated plantPreparation of sample solution from regenerated plant Solution heated on for 20mins in water bath N.B. : Following test are done by this solution Solution heated on for 5 mins in water bath Half of them absorved by alcohol and other s absorbed by water for 24 hrs.
  • 40. Test of Market sample Culture sample observation conclusion Eth solution Aq solution Eth solution Aq solution pholobatannin s Sample+ 1%HCl Sample+ 1%HCl Red ppt are found pholobatanni ns Present Flavonoid Sample+conc.H 2SO4+5ml NH4OH Sample+conc.H 2SO4+5ml NH4OH Yellow color appeared Flavonoid Are present Steroid 2 ml Acetic anhydride+0.5 ml sample+2ml H2SO4 2 ml Acetic anhydride+0.5 ml sample+2ml H2SO4 Violet blue green color appeared Steroid are present Terpinods Sample+2mlCH 3Cl+conc.H2SO4 Sample+2ml CH3Cl+conc.H2S O4 Radish brown color Terpinodes are present Cardiac glycoside 2ml glacial acetic acid +ferric chloride solution+extrac t+conc H2SO4 2ml glacial acetic acid +ferric chloride solution+extrac t+conc H2SO4 Brown ring formation Cardiac glycoside are present Amino acid Sample +few drops ninhydrin+wat er bath heating Sample +few drops ninhydrin+wat er bath heating Violet color Amino acid are present
  • 41. Test of pholobatannins: Sample solution +1%HCl= ๏‚ง Red ppt are found Pholobatannins test Flavonoid test Test of flavonoid Sample+conc.H2SO4+ 5ml NH4OH = Yellow color appeared
  • 42. โ€ข Test of Steroid 2 ml Acetic anhydride+0.5ml ethanolic sample solution+2ml H2SO4 =Violet blue green color appeared and ring formation โ€ข Test of Terpinoid โ€ข Sample+2mlCH3Cl+conc. H2SO4 = Radish brown color
  • 43. โ€ข Test of cardiac glycoside โ€ข 2ml glacial acetic acid +ferric chloride solution+extract+conc H2SO4 = yellow color appeared โ€ข Test of amino acid โ€ข Sample +few drops ninhydrin+water bath heating = Violet color appeared
  • 44. 1.0 mg/l of BAP &1.0mg/l of NAA gave the best result for in vitro shoot formation. The study showed addition of 1mg/l IBA gave profuse of rooting. The similarity in the Phytochemichal analysis in both regenerated and control one for pholobatannins, cardiac glycoside, Steroid , Terpinoid and amino acid showed a possibility of using these regenerated plants for other uses. A quick and easy micropropagation protocol of the medicinal plant Bacopa monnieri has been established ConClusion
  • 45.
  • 46. โ€ข Glycosides of 20-deoxy derivatives of jujubogenin and pseudojujubogenin from Bacopa monniera. , Planta Med. 2011 ;73(4):380-3. Neuroprotective role of Bacopa monnieri extract in epilepsy and effect of glucose supplementation during hypoxia: glutamate receptor gene expression.G. Phani Kumar and Farhath Khanum, Pharmacognosy Rev. (2012) 6(12) 81-90. Ayurvedic medicinal plants for Alzheimer's disease: a review Rammohan V Rao, Olivier Descamps, [., and Dale E Bredesen Alzheimer's Res. Ther. (2012) 4(3):22 Singh RH, Narsimhamurthy K, Singh G Neuronutrient impact of Ayurvedic Rasayana therapy in brain aging. Biogerontology. 2008 Dec;9(6):369-74. doi: 10.1007/s10522-008-9185-z.
  • 47. Kulhari A1, Sheorayan A1, Bajar S2, Sarkar S3, Chaudhury A1, Kalia RK1. Investigation of heavy metals in frequently utilized medicinal plants collected from Springerplus. 2013 Dec 17;2:676. doi: 10.1186/2193-1801-2-676. Srivastava P, Raut HN, Puntambekar HM, Desai AC. Stability studies of crude plant material of Bacopa monnieri and quantitative deter Phytochem Anal. 2012 Sep-Oct; 23(5):502-7. Doi: 10.1002/pca.234 Williams R, Mรผnch G, Gyengesi E, Bennett L. Bacopamonnieri (L.) exerts anti-inflammatory effects on cells of the innate immune Food Funct. 2014 Jan 22.
  • 48. I AM MOST THANKFUL TO PROF.A.CHAKRAVARTHY DR.SUDIPA CHAKRAVARTHY DR.MADHUMITA.J.MUKHOPADHYA AND DEBRAJ SIR FOR HELPING ME WITH THIS PROJECT.