ISOLATION OF GENOMIC DNA FROM PLANT TISSUE

 ISOLATION OF GENOMIC DNA

        Isolation of  DNA from the plant tissues is at the heart of      plant molecular biology.   

GENOME :
                 The sum of total of all genetic material of an organism, which stores biological information are called genome.
                 The nature of DNA may be either DNA or RNA.

AIM:
             To isolate DNA from the given sample and quantify the                    DNA.

PRINCIPLE: 
              
             The basic step of DNA isolation are disruption and lysis of cellular structure & separation of the  soluble DNA followed by the removed of protein & outer cell concentration.The concentration of isopropanol will cause the DNA to become insoluble since DNA molecules are ionic.They are highly soluble in water & ethanol are commonly used to precipitate DNA from aqueous solution.

                         
                                

REQUIREMENTS:
              
           - Plant sample (Acalypha indica) ,
           - Extraction Buffer,
           - Centrifuge,
           - Chloroform,
           - Isoamyl alcohol, 
           - Isopropanol,
           - TE Buffer.

EXTRACTION BUFFER PREPARATION :
          
           0.5 M EDTA  PH - 8.0          - 10 ml
           1 M Tris Hcl  PH - 7.4         -  4  ml
           5 M Nacl                               - 28 ml
           Makeup Dis.H20 100 ml    - 58 ml
           0.2 % beta - Mercaptoethanol  - 1  ml


PROCEDURE :
           

•  About 1 g of  fresh leaves was weighed & ground well with 5 ml of extraction buffer and add 2 % w/v CTAB mixed gently (do not stir).

• The sample was given gentle inversions & the homogenate was incubated in a warm water bath maintained at 65*C for 1 hour.  

•  After incubation , the homogenate was brought to room temperature and centrifuged at 10,000 rpm for 10 minutes at room temperature.

• Then , the extract was pipetted out into a sterile 15 ml falcon tube. 

                                    

•    The extract with equal volume of chloroform: Isoamyl               alcohol (24:1) & centrifuged at 8,000 rpm for 10 minutes at       room temperature.

•    After centrifugation the resultant recover the top aqueous           phase was transferred to a new sterile falcon tube and  add         0.7 ml /L volume of isopropanol & mix gently.

•   The sample was given incubation at -20*C for 30 minutes &      then centrifuged at 10,000 rpm for 10 minutes at 4*C.

•    Finally DNA pellet was obtained by decanting the                     supernatant followed by washing with ethanol.

•    The pellet was air dried till the ethanol had evaporated.

•   The air dried pellet was re-suspended  in 0.1 ml of TE                buffer & stored at -20*C for further use.

  Thus the genomic DNA was observed under UV- transilluminator.







               

     ANOMALOUS SECONDARY GROWTH

                        NYCTANTHUS

• It belongs to the family Nyctanthaceae.
• Epidermis is single layered and it is cuticularized by a thick cuticle.
• Many multi-cellular hairs are present.
• Epidermis is followed by the cortex which is few layered & it is differentiated into collenchyma and  parenchyma cells.
• Parenchyma is found below the collenchyma.
• Below that, cortical bundles (vascular bundles) are present, which are 4 in number respectively.
• They are con-joint,collateral,open and exarch.
• Below the cortical bundles, cambium is found as single-layered.
• Here the phloem found outwards, xylem towards inwards & in between cambium is present.
• Endodermis is single layered and not so developed well.
• Pericycle is found in the form of sclerenchymatous patches.
• Primary phloem is crushed & irregularly present in patches below pericycle.

ANOMALOUS SECONDARY GROWTH:
ABNORMALITIES:

       Here, the presence of vascular bundles in the cortex region is the anomalous growth, which are found inversely oriented , and they are never connected to the main ring of the vascular cylinder.

Anomalous secondary growth

             SECONDARY GROWTH IN DICOT STEM

                                         BIGNONIA

    

                      Bignonia, is a member of Bignoniaceae family & it is a dicotyledonous plant. It was a woody climber. In that , young stem shows ridges & furrows.

In transverse section, bignonia shows following anatomy,such as :

   

                        

                   

EPIDERMIS: 

• It is the outermost layer of the rectangular cells .
• Thick cuticle is present over the upper layer of the epidermis.

HYPODERMIS:

• Beneath the epidermis,few layered collenchymatous  hypodermis cells are present in the ridges and furrrows.
• Chlorenchyma cells may also be present.

CORTEX:

•  A single layered cortex acts as endodermis, and also contains    inter cellular spaces. 
•  And the cells are without casparian thickenings.

PERICYCLE:

•  It is made up of  alternate bands of sclerenchyma cells with  parenchymatous tissues.    
• Pericycle is not continuous , present like patches.

VASCULAR BUNDLES:

•   Vascular bundles are arranged in the form of ring and they         are collateral,con-joint,open & with endarch xylem.
•   Secondary phloem present below the pericycle.
•   Cambium as single-layered.
•   Medullary rays made partition of sclerenchymatous patches.

ANOMALOUS SECONDARY GROWTH:

• Phloem growth is higher in rate , so the presence of medullary rays makes the phloem pulls inwards, this may makes like wedge-shaped phloem.

                             

• While the secondary phloem & secondary xylem present upside and primary phloem & secondary xylem present below then disappears as faster as faster respectively.

  FUNGAL DISEASES & THEIR CAUSATIVE ORGANISMS

WHITE RUST OF MUSTARD & CRUCIFERS :     Albugo candida        (CLASS : Oomycetes ) 

BLIGHT OF CRUCIFERS                                    :    Alternaria brassicae (CLASS : Deutromycetes)

CLUB ROOT OF CRUCIFERS                            :    Plasmodiaphoria brassicae   (Deutromycetes)

DOWNY MILDEW OF CRUCIFERS                  :   Peronospora parasitica          (Oomycetes)

STEM OR FOOT ROT OF PAPAYA                    :   Pythium aphanidermatum       (Oomycetes)

RHIZOME & ROOT ROT OF TURMERIC       :   Pythium aphadermatum         (Oomycetes)

LEAF SPOT OF TURMERIC                               :   Taphrina maculans                 (Ascomycetes)

LEAF RUST OF COFFEE                                     :   Hemileia vastatrix                 (Basidiomycetes)

STEM RUST OF WHEAT                                      :  Puccinia graminis tritici        (Basidiomycetes)

YELLOW RUST OF WHEAT                               :  Puccinia striiformis               (Basidiomycetes)

LOOSE SMUT OF WHEAT                                  :  Ustilago nuda                        (Basidiomycetes)

 

LOOSE SMUT OF BARLEY                                :  Ustilago nuda                        (Basidiomycetes)

COVERED SMUT OF OAT                                  :  Ustilago kolleri                      (Basidiomycetes)

RUST OF MAIZE                                                   :  Puccinia sorghi                     (Basidiomycetes)

WILT OF BANANA                                                :  Fusarium cubense

WILT OF FLAX                                                      :  Fusarium lini

WILT OF GRAM                                                    :  Fusarium ortaceros

WILT OF ARHAR & PIGEON PEA                    :  Fusarium odum

RED ROT OF SUGARCANE                                : Colletotrichum  falcatum      (Deutromycetes)

 

                

      PLANT DISEASES & CAUSATIVE ORGANISMS

                              BACTERIAL DISEASES

• BACTERIAL WILT OF POTATO                       :     Pseudomonas  solanacearum
• RING ROT OF POTATO                                       :     Cornyebacterium  sepedonicum
• CITRUS CANKER                                                  :      Xanthomonas citri
• BACTERIAL STRIPE OF SORGHUM             :      Pseudomonas andropogoni
• BACTERIAL STREAK OF SORGHUM           :     Xanthomonas holcicola 
• BACTERIAL LEAF SPOT OF SORGHUM     :     Pseudomonas syringae
• LEAF SPOT OF PEARL MILLET                      :    Xanthomonas penniseti 
• BLIGHT OR SPOT OF LEAF MILLET            :     Pseudomonas alboprecipitans 
• BROWN STRIPE OF FINGER MILLET         :     Pseudomonas setariae 
• FIRE BLIGHT OF APPLE & PEAR                  :     Erwinia amylovora 
• BACTERIAL BLIGHT OF RICE                        :     Xanthomonas oryzae 

                                                  

                          

BASICS & PROCEDURES OF PLANT TISSUE CULTURE TECHNIQUES

                                              

                                                BASICS OF PLANT TISSUE CULTURE

                      Tissue culture is the method of “in vitro” culture of plant or animal cells, tissue or organ grown on nutrient medium under aseptic conditions usually in   a glass container.  It   is   sometimes referred   to as ‘sterile culture’ or ‘in vitro’ culture.

 By this technique living cells can be maintained outside the body of the organism for considerable period. Tissue culture involves both plant and animal cells, tissue culture produces clones, in which all product cells have the same genotype.

                      A more recent advance is the use of plant and animal tissue culture along with genetic modification using viral and    bacterial vectors and gene guns to create   genetically   engineered organisms.

                                          


                                       

             

                   
   

  

 INTRODUCTION:

     

                            Plant tissue culture is a method or technique to isolate parts of plants (protoplasm, cells, tissues, and organs) and grow them on artificial media in aseptic conditions in a controlled space so that parts of these plants can grow and develop into complete plants.

                            It is a collection of techniques used to maintain or grow plant cells, tissue or organ, under sterile condition on a nutrient culture medium of known composition.

                      

                            There are numerous methods to propagate plants in tissue culture, but the one principle that is Constant (ie.) totipotency.

               

WHAT IS TOTIPOTENCY ?

                   

                        The property of a normal cells that they have the genetically potential or capacity to give rise to a completely new individual plant species, referred as totipotency.

                     This is because every cell has the genetic potential of the parent plant, the basic steps starts with the regeneration of whole plants from an explants or cell.

WHAT IS EX- PLANT  ?

                       

                          It is referred as that the any portion or a piece of a plant material which can be used in a cultured medium to establish   a tissue culture system or to regenerate a new whole plant.

                                                                                                            

WHAT IS CALLUS ?

                       

                     It is referred to as undifferentiated mass of cells.
             

                                               

                                                                                      

PROCEDURES OF PLANT TISSUE CULTURE :

                     Preparation of instruments and nutrients culture medium

                     Sterilization of culture medium

                     Preparation of Explant

                     Inoculation of Explant

                     Incubation for growth

                     Acclimatization of plantlets & Hardening

Preparation of instruments and nutrient medium :

             

·         The area dedicated to media preparation should comprise of sufficient storage space for the chemicals, culture glassware/vessels etc.

·         And the lab procedures and rules should be followed strictly to maintain aseptic conditions respectively.

·         The media room should be maintained with cleanliness, removal of contaminated cultures, restricted entry.

        Thus, a sterile area is required for performing various aseptic manipulations during tissue culture.  In other hand we can see about the preparation of instruments, required for the plant tissue culture techniques.

APPARATUS REQUIRED :

·         Forceps

·         Scissors

·         Blade holders

·         Disposable and surgical blades

·         Petri plates with 2 filter papers

·         500 ml beaker

·         350 ml Erlenmeyer flask

·         500 ml test tubes

·         Disposable pipette tips

·         Pipettes and 100 ml bottle with screw cap

1.       Apparatus are trapped in newspaper or brown paper to undergo autoclaving for an hour.

2.       Before the process of plant tissue before using culture, it is required to sterilizes and clean the vessels respectively.

3.       Before using any glass wares for any culture preparation, they are cleaned in 4 steps processes, as given below.

4.       Al glass wares & plastic wares should be autoclaved for an hour.

5.       And, all wares were immersed in tub-full of promic acid for 16 hours.

6.       Then it is washed or rinsed in water to remove the promic acid.

7.       After this, all glass wares & plastic wares are immersed and washed in detergent water with a hard nylon brushes.

8.       Then the glass wares & plastic wares are immersed and cleaned in other tub-full of clean water, the detergent is rinsed off.

9.       Finally the glass wares & plastic wares are cleaned in the running tap water & kept in clean trays then place into the oven with temperature of 60-80*c for drying process.

10.   Thus the dried glass wares are now ready for use.

 PREPARATION OF CULTURAL MEDIUM:                        

                             

                                       

                                         

                                   

           

•   Growing of desirable micro-organisms in a nutrient medium is known as medium.

•         Thus the next important method is preparation of media, which is used in micro propagation techniques.

                                                                                                                                                      

•       Media, here used is composed of group of micro and macro elements, vitamins, amino acids (glycine) and mostly sucrose, which serves as a main source of carbon and carbohydrates for the plant.
• 
  
•          The amount of elements used are weighed accurately as per the reported formulations and dissolved in de-ionized water to avoid the precipitation of salts and it prevents the availability of salts to the plants.
• 
  
•           Here, the salts with higher solubility dissolves first, generally the plants can takes the                 nutrients, ranges from PH 5.6-5.8.
• 
  
•                   After the medium at ranges the desired PH, it is ready to be poured in 250ml of Erlenmeyer       flask or 50ml test tubes as 100ml / 20ml.
• 
  
•                 Semi-solid medium as to be prepared, so take 0.75 mg -0.8mg of Agar-Agar, this amount            provide optimum solidification and moisture content to the culture.

•         100ml of medium is carefully poured into the each 250ml of Erlenmeyer flask and plucked       with non- absorbent cotton plucks, covered with muslin- cotton at the opening top of the flask,   for easy holding of the cotton plucks. 

STERILIZATION OF CULTURAL MEDIUM:

·         Sterilization is a method of removal of unwanted microbes from the desirable cultural medium. It can be done by following methods,

                                                               

v  Sterilization by moist heat

                                                 

v  Sterilization by dry heat

v  Surface sterilization

STERILIZATION BY MOIST HEAT:
AUTO CLAVING:        

                                 

                                     

Ø  Autoclave is a device used to sterilize the instruments by means of moist heat such glass wares, cultured media with high- pressure saturated steam.

Ø    Autoclave the media for 20 minutes at high temperature of 120*C and pressure 15 pascal.

 PREPARATION OF EX-PLANTS :

                                 Different kinds of explants such as leaves , petals, buds, ovaries , seeds, anthers and nodal segments can be used in tissue culture because , each & every cells of the cells of the plants are eligible to give rise to the new plants of individuals.

However it should be carefully to collect the plants as,

• Disease -free,
• Healthy & actively growing plants,                  

Immediately , after collections , the explants are placed in clean-water to avoid air-bubbles , microbes and contaminants from the cut - exposed plant parts.

And to avoid browning , due to the phenolic oxidation.

This explants are brought to the lab for  the further sterilization processes.

                                       

                                       
                                     

First, this explants are cut into small pieces with the help of sterilized scissors, and then placed in a petri-plate containing a clean water.

The surface of the ex-plants are brushed clean with stable-hair brush to make it light-wet.

And all the small pieces of cut- explants were placed into a plastic - wares of containing the mild solution of fungicides as an antibiotic respectively.

Then, the pieces of the ex-plants are cleaned & rinsed well with a clean & de-ionized water.

Finally the ex-plant pieces are immersed in a clean de-ionized water and then taken to the inoculation chambers.

INOCULATION OF EX-PLANT :

                  While entering the inoculation chamber, it is neccessary to wear a clean cotton lab-coat.

                  Inoculation means transfer of plant specimen to the media under a septic conditions.



PREPARATION OF LAMINAR HOOD: 

                                

•  Laminar hood is a special equipment for inoculation processes.  
•  Shud the shutter of the laminar-hood  switch on the UV light for about 30 minutes.
•  UV eyes can kill all microbes, it is highly dangerous to human eyes and skin.      
•   Before  switching off the UV lights, the shutter should not be opened.
•  After 30 minutes, switch off the UV lights and switch on the chamber lights with the shutters  opened.
•  And switch on the laminar - hood.
• While operating laminar-hood , it is neccessary to wear  headmask and face masks.
• And use hand wash (detol) for hand in sterile conditions.
• The Ex-plants are washed with 70% of ethanol for few seconds and then treated with mild mercuric chloride solution for a few minutes.
• And keep the open mouth of the conical flask near to the spirit lamp to avoid the invasion of any other microbes.
• Keep on mind that,generally use a mild solution for longer duration, and use strong solution for short duration.
• After the sterilization process, the solution is decanted into the another beaker, then the Ex-plants are  washed several times after and after to remove the mercuric chloride solution.
• Now, after cooling the forceps, before treated with 70% ethanol , used to transfer the ex-plant pieces from conical flask to the petri-plate.
• Before this the petri-dish is placed to sterilized above the spirit -lamp to avoid microbial invasions.
• Place the ex-plants over  the filter paper placed over the petri-plate, were it absorbs the excess amount of water.
• The ex-plants which are exposed to the mercuric chloride are removed with blades.

• Each nodal-segments were carefully taken and transferred to the test tubes containing media.
• It is very important that forceps could not touches the rim of the test tube and mainly the media.

• After that the cap is put tightly over the test tube and sealed well..

• Finally, name of the plant, date of inoculation were labelled over the surface of the test tube.

• The culture are now ready to be inoculated.
•  At optimum conditions, with 16 hours light alternating with 8 hour darkness, at 25-27                degree Celsius  temperature and 40% relative humidity and it is monitered alternately.

• The time of culture grows starts from 12-15 days without any bacterial or fungal                          contaminants.

•  And the corresponding cultures are allowed to grow respectively.

•  And a period of time they arises like shoot developed in conditions.

•  Once , the shoot is grown at the appreciable height(3-4 cm).
•  Generally , auxins are used in culture medium .

•  Once they are grown well in the lab conditions, they are ready for acclimatization .

 

ACCLIMATIZATION OF PLANTLETS &TRANSFER TO POTS :

                            

                                         

   

•     Now the tissue cultured plantlets are transferred to green house condition.
•     Green houses normally has decreased relative humidity , intensity and aseptic conditions.
•     And when the plantlets reaches 3-4 inches, transfer them into a  new pots consists of               garden  sand,soil,well decomposed farm yard manure at the  ratio of 1:1:1.
•     After 45-60 days, these acclimatized plants can be shifted to the outer door conditions.

                                                  

                                              

                                              

Thus , plant tissue culture plays a major role in production of transgenic and disease free resistance plants such as  Bt Cotton, Amentotaxus assamica, Lotus corniculatus, Psilotum nudum . And also used in the used in the yielding of medicinal plants , also in the food industries,..                                   

  

                                                              

                                                                    THANK YOU