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Transcript of Summer Training Reprt Best Biotech
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LABORATORY
RULES
There are some rules which must be observed form the successful
completion of the laboratory exercise, personal safety convenience of others
working in the laboratory.
1)Always wear a laboratory coat or apron before entering a laboratory for
protecting clothes form contamination or accidental discoloration by
staining solution.
2)Before and after each laboratory period clean your workbench with
disinfectant like Lysol (1; 500) phenol (1; 100) or 90% ethanol.
3)Keep your laboratory bench clean of everything (e.g. Books, purses,
papers, etc.) Except your laboratory equipment and notebook.
4) Never smoke, drink or eat in the laboratory.
5) Never place pencil, labels or any other material in your mouth.
6)If a live cultured spilled, cover the area with a disinfectant such as
mercuric chloride for 15 min and then clean it.
7)In the event of personal injury such as cut or burn, inform your
constructor immediately as bacteria love open wounds.
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8)Long hair should be tied back to minimize contamination of cultures and
fire hazards.
9)Be careful of laboratory burners and turn them off when not in use.
10) All microbial cultures should be handled as being potential
pathogenic.
11) The waste papers and contaminated glassware’s should be kept in
recepecticals provided.
12) Wash your hands with soap and water before and after finishing
work in the laboratory.
13) Broth cultures must never be pipitted with mouth and must be
filled with the use of pipette aids and operated in such a way so as to
avoid creating aerosol.
14) Aseptic technique must be rigorously observed at all times.
15) Always culture tubes in an upright position in a rack or basket.
16) You must familiarize yourself in advance with the excise to be
performed.
17) Label all the plate’s tubes, cultures properly before starting an
exercise to be performed.
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IMPORTANCE OF MICROBES
Beneficial
Microbes are used to make vaccines (attenuated or weak/dead microbes), which can be injected or
inoculated into a host organism to stimulate the production of blood substances (called antibodies) to
insure future protection against the possible contact with an unwanted microbe. Vaccines are most often
produced by using attenuated viruses or bacteria. Later in the course we will discuss vaccination series
such as MMR and DPT. A second important medical use of microbes involves the production of
antibiotics like penicillin and bacitracin. Antibiotics are molecules produced by bacteria and molds (or
talented chemists) that can be injected, taken orally, or occasionally used topically to inhibit new growth
of bacteria. Transferring genes (usually by a loose strand of DNA called a plasmid) cells can be directed
to produce needed substances like insulin and erythropoeitin (hormone needed for development of red
blood cells). This bio-engineering is an exceptionally important use of microbes in modern science.
Students in agronomy (plant technologies) and soil science may know that genes from
bacteria like Agrobacterium can be used in bio-engineering to develop disease resistance in plants. Also
soil microbes are helpful in breaking down (decomposition) of dead organic material in the soil resulting
in addition of nutrients to the soil. Still other soil microbes release minerals that are attached to soil
particles and/or fix nitrogen. Since most nitrogen is in the atmosphere and not available to plants,
microbes must combine the nitrogen with oxygen to make a soluble molecule called a nitrate which can
be taken in through the roots.
During the breakdown of carbohydrates by microbes, numerous products like acids and
alcohols may be produced. The production of these chemicals is a major industrial use of microbes. In
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the fermentation process, many foods including cheese and silage (animal food often used in the dairy
industry) are the result of microbe activity. Pasteur was an early microbiologist who studied
fermentation of grapes resulting in the production of wine. Later he introduced pasteurization (heating)
to eliminate additional microbial fermentation so the wine "did not go bad." Saccharomyces (yeast) and
Zygomonas (a bacterium) are commonly used to make beer and tequilla respectively.
Microbes are also important in environmental studies. The breakdown of sewage and oil
slicks (spills) returns the environment to its desired original condition. This return to the original
environment is called bio-remediation. In the food chains of nature, microbes are often one of the early
sources of energy needed to maintain the community. Microscopie algae convert sunlight into useable
food and small protozoans and bacteria serve as a primary (bottom) step in food chains. This
microscopic plankton is essential ion water communities.
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Indu strial microbiology
Industrial microbiology encompasses the use of microorganisms in the manufacture of food or industrial products. The use of microorganisms for the production of food, either human or animal, is
often considered a branch of food microbiology. The microorganisms used in industrial processes may be natural isolates, laboratory selected mutants or genetically engineered organisms.
Industrial Application of microbes
Food microbiology
Yogurt, cheese, chocolate, butter, pickles, sauerkraut, soya sauce, vitamins, amino acids, food thickeners
(microbial polysaccharides), alcohol, sausages, and silage (anima food) are all produced by industrialmicrobiology processes. "Good" bacteria such as probiotics are becoming increasingly important in the
food industry.
Biopolymers
A huge variety of biopolymers, such as polysaccharides, polyesters, and polyamides, are produced by
microorganisms. These products range from viscous solutions to plastics. The genetic manipulation of
microorganisms has permitted the biotechnological production of biopolymers with tailored material properties suitable for high-value medical application such as tissue engineering and drug delivery.
Industrial microbiology can be used for the biosynthesis of xanthan, alginate, cellulose, cyanophycin, poly(gamma-glutamic acid), levan, hyaluronic acid, organic acids, oligosaccharides and polysaccharides, and polyhydroxyalkanoates.
Bioremediation
Microbial biodegradation of pollutants can be used to cleanup contaminated environments. These
bioremediation and biotransformation methods harness naturally occurring microbes to degrade, transform or accumulate a huge range of compounds including hydrocarbons (e.g. oil), polychlorinated
biphenyls (PCBs), polyaromatic hydrocarbons (PAHs), pharmaceutical substances, radionuclides and
metals.
Waste biotreatment
Microorganisms are used to treat the vast quantities of wastes generated by modern societies.
Biotreatment, the processing of wastes using living organisms, is an environmentally friendly, relatively
simple and cost-effective alternative to physico-chemical clean-up options. Confined environments,such as bioreactors] can be employed in biotreatment processes.
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Health-care and medicine
Microorganisms are used to produce human or animal biologicals such as insulin, growth hormone, andantibodies. Diagnostic assays that use monoclonal antibody, DNA probe technology or real-time PCR
are used as rapid tests for pathogenic organisms in the clinical laborarory.
Archaea
Examination of microbes living in unusual environments (e.g. high temperatures, salt, low pH or
temperature, high radiation) an lead to discovery of microbes with new abilities that can be harnessed
for industrial purposes.
Corynebacteria
Corynebacteria are a diverse group Gram-positive bacteria found in a range of different ecological
niches such as soil, vegetables, sewage, skin, and cheese smear. Corynebacterium glutamicum is of immense industrial importance and is one of the biotechnologically most important bacterial specieswith an annual production of more than two million tons of amino acids, mainly L-glutamate and L-
lysine. The genome sequence of C. glutamicum has been published
Harmful
Earlier we stated that most microbes are beneficial; however, some microbes do damage and are
potentially harmful and costly. Some microbes cause disease and are called pathogens. Early
microbiologists like Louis Pasteur and Robert Koch completed experiments showing that diseases could
arise when microbes entered and grew in tissues. Between 1875 and 1900 Robert Koch found the
causative microbes of at least 20 diseases. This germ theory of disease, which identifies the cause of
disease- “one microbe, one disease”, is still used and important today.
Large populations of microbes may also cause infestations thus reducing the potential productivity of
host organisms. Examples of microbes that infest other living organisms include roundworms or
nematodes, flukes, tapeworms, and spider mites. These ectoparasites (on surface) and endoparasites
(inside host) may infest as many as 50 million people annually in our country. If bacteria increase in
high numbers in water, oxygen is depleted and many living organisms like fish may die form lack of
oxygen.
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The presence of microbes also may indicate spoilage. It is estimated that 30% or more of all food
produced in our country may be lost to spoilage. The change in color, texture, or smell of the food
makes the food less palatable and therefore is often discarded. Spoilage of food is defined as food
discarded because of the presence of microbes and/or toxins (poisons) released in to the food.
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Isolation and enumerationof Bacteria form Soil
Sample
PURPOSE
Isolation and enumeration of microorganisms from soil sample .
MATERIALS
Cotton swabs, nutrient agar media, 3 petri plates, 6.test tubes, magnetic shaker, pipette, distelled water,
colony counter, 1.conical flask.
COMPOSITION OF NUTRIENT AGAR. (100 ML)
• Peptone ------ .5g
•
• Beef extract 3g
•
• NaCl 5g
•
• Distelled water 100ml
•
• Agar 2g
METHOD USED-- SERIAL DILUTION AGAR-PLATING METHOD
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FORMULA USED
No of cells per g of soil = (mean plate count *dilution factor)/dry wt of soil.
PRINCIPLE
NO of colonies developed = no of microorganism in the media
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EXPERIMENTAL PROCEDURE
10ml sterile distilled water was taken in a test tube. Take 1gm of soil sample and dissolve in the
first test tube.. The tube was vigorously vortexed for 3 minutes to obtain uniform suspension of
microorganisms.
A series of tubes, labeled as 10-1, 10-2 to 10-7, were filled with 9ml sterile distilled water. 1ml of
diluted sample was transferred to the tube marked 10 -1 and vigorously vortexed. 1ml from this
tube was transferred to the tube marked as 10-2 and vigorously vortexed.
The process was repeated up to 10-7.
Pour plate method was used to culture Bacteria using Nutrient Agar media. Three sterile Petri
plates were taken and labeled as 10-2, 10-3, and 10-4.
To this 1 ml aliquots each from 10-2, 10-3, and 10-4 serial dilution were transferred to respective
pertiplates.
Then approximately 15ml of cooled (450 C) starch agar medium was added to each Petri plate
and the inoculums was mixed by gentle rotation of Petri plates.
After solidification of medium the plates were incubated for 24 hours at 370C.
OBSERVATION
After incubation bacterial colonies were developed in all the Petri plates.
First two Petri plates were highly covered with bacterial colonies so unable to count.
Third Petri plate contains countable number of colonies.
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Number of colonies counted were = 71
VIABLE COUNT
10-1 dilution:
10-2 dilution:
10-3 dilution:
10-4
dilution:
10-5 dilution:
10-6 dilution:
ENUMERATION OF MICROORGANISMS BY VIABLE COUNT
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CALCULATION
No of cells per g of soil = (mean plate count *dilution factor)/dry wt of soil
= ( 71 * 10^6)/0.8
=
RESULT
The number of cells per gram of soil=
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TECHNIQUE FOR ISOLATION OF PURE CULTURES:
Mature, microbial populations do not segregate themselves by species but exist with a mixture of any other cell types. In the laboratory, these populations can be separated into pure cultures. These
cultures contain only one type of organism which is suitable for the study of their cultural,
morphological, and biochemical properties.
In this experiment, technique is designed to produce discrete colonies. Colonies are
individual, macroscopically visible masses of microbial growth on a solid medium surface, each
representing the multiplication of a single organism. Once stained these discrete colonies, we will make
aseptic transfer onto nutrient agar slants for isolation of pure cultures.
AIM
Perform the spread-plate and/or the streak-plate inoculation procedure for the separation
of the cells of a mixed culture so that discrete colonies can be isolated.
PRINCIPLE
The techniques commonly used for isolation of discrete colonies initially require that the number
organisms in the inoculum be reduced. The diminution of the population size ensures that, following
inoculation, individual cell will be sufficiently far apart on the surface of the agar medium to effect a
separation of the different species present. The following are techniques that can be used to accomplish
this necessary dilution.
The streak-plate method is a rapid qualitative isolation method. It is essentially a dilution
technique that involves spreading a loopful of culture over the surface of an agar plate. Although many
types of procedures are performed, the four-way, or quadrant, streak is described.
PROCEDURE:
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• Place a loopful of culture on the agar surface in Area 1. Flame and cool the loop and drag it
rapidly several times across the surface of Area 1.
• Reflame and cool the loop and turn the Petri dish 90°. Then touch the loop to a corner of the
culture in Area 1 and drag it several times across the agar in Area 2. The loop should never enter
Area 1 again.
• Reflame and cool the loop and again turn the dish 90°. Streak Area 3 in the same manner as
Area 2.
• Without reflaming the loop, again turn the dish 90° and then drag the culture from a corner of
Area 3 across Area 4, using a wider streak. Don’t let the loop touch any of the previously
streaked areas. The flaming of the loop at the points indicated is to effect the dilution of the
culture so that fewer organisms are streaked in each area, resulting In the final desired
separation.The spread-plate technique requires that a previously diluted mixture of microorganisms be used.
During inoculation, the cells are spread over the surface of a solid agar medium with a sterile, L-shaped
bent rod while the Petri dish is spun on a “lazy-Susan” turntable. The step-by-step procedure for this
technique is as follows:
• Place the bent glass rod into the beaker and add a sufficient amount of 95% ethyl alcohol to
cover the lower, bent portion.
• With a sterile loop, place a loopful of M. luteus culture in the center of the appropriately labeled
nutrient agar plate that has been placed on the turntable. Replace the cover.
• Remove the glass rod from the beaker and pass it through the Bunsen burner flame, with the bent
portion of the rod pointing downward to prevent the burning alcohol from running down your
arm. Allow the alcohol to burn off the rod completely. Cool the rod for 10 to 15 seconds.
• While the Petri dish cover and spin the turntable.
• While the sterile bent rod to the surface of the agar and move it back and forth. This will spread
the culture over the agar surface.
• When the turntable comes to a stop, replace the cover. Immerse the rod in alcohol and reflame.
The pour-plate technique requires a serial dilution of the mixed culture by means of a loop or
pipette. The diluted inoculum is then added to a molten agar medium in a Petri dish, mixed, and
allowed to solidify.
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BACTERIAL STAINING
WHAT ARE BACTERIA?
Until recently, the term bacteria were used for all microscopic prokaryotes. But, it turns out that there
are two groups of prokaryotes that differ from each other in just about every way except size and lack of
a nucleus. These are now distinguished as the:
• Bacteria; the "true" bacteria (also known as Eubacteria)
• Archaea; (also known as Archaebacteria)
The archaea are so different from the bacteria that they must have had a long, independent evolutionary
history since close to the dawn of life. In fact, there is considerable evidence that you are more closely
related to the archaea than they are to the bacteria!
PROPERTIES
•Prokaryotic (no membrane-enclosed nucleus)
• No mitochondria or chloroplasts
• A single chromosome
o A closed circle of double-stranded DNA
o With no associated histones
• If flagella are present, they are made of a single filament of the protein flagellin; there are none
of the "9+2" tubulin-containing microtubules of the eukaryotes.
• Ribosome’s differ in their structure from those of eukaryotes
• Have a rigid cell wall made of peptidoglycan.
• The plasma membrane is a phospholipid bilayer but contains no cholesterol or other steroids.
• no mitosis
• Mostly asexual reproduction
• Any sexual reproduction very different from that of eukaryotes; no meiosis
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• Many bacteria form a single spore when their food supply runs low. Most of the water is
removed from the spore and metabolism ceases. Spores are so resistant to adverse conditions of
dryness and temperature that they may remain viable even after 50 years of dormancy.
CLASSIFICATION
Until recently classification has done on the basis of such traits as:
• Shape
o Bacilli: rod-shaped
o Cocci: spherical
o Spirulla: curved walls
• Ability to form spores
• Method of energy production (glycolysis for anaerobes, cellular respiration for aerobes)
• Nutritional requirements
• Reaction to the Gram stain.
Although the Gram stain might seem an arbitrary criterion to use in bacterial taxonomy, it does, in fact,
distinguish between two fundamentally different kinds of bacterial cell walls and reflects a natural
division among the bacteria.
More recently, genome sequencing, especially of their 16S ribosomal RNA (rRNA), has provided new
insights into the evolutionary relationships among the bacteria.
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GRAM STAIN
HISTORY AND HOW IT WORKS
The Gram staining method, named after the Danish bacteriologist who originally devised it in 1844,
Hans Christian Gram, is one of the most important staining techniques in microbiology. It is almost
always the first test performed for the identification of bacteria. The primary stain of the Gram's method
is crystal violet. Crystal violet is sometimes substituted with methylene blue, which is equally effective.The microorganisms that retain the crystal violet-iodine complex appear purple brown under
microscopic examination. These microorganisms that are stained by the Gram's method are commonly
classified as Gram-positive or Gram non-negative. Others that are not stained by crystal violet are
referred to as Gram negative, and appear red.
Gram staining is based on the ability of bacteria cell wall to retaining the crystal violet dye during
solvent treatment. The cell walls for Gram-positive microorganisms have a higher peptidoglycan and
lower lipid content than gram-negative bacteria. Bacteria cell walls are stained by the crystal violet.
Iodine is subsequently added as a mordant to form the crystal violet-iodine complex so that the dye
cannot be removed easily. This step is commonly referred to as fixing the dye. However, subsequent
treatment with a decolorizer, which is a mixed solvent of ethanol and acetone, dissolves the lipid layer
from the gram-negative cells. The removal of the lipid layer enhances the leaching of the primary stain
from the cells into the surrounding solvent. In contrast, the solvent dehydrates the thicker Gram-positive
cell walls, closing the pores as the cell wall shrinks during dehydration. As a result, the diffusion of the
violet-iodine complex is blocked, and the bacteria remain stained. The length of the decolorization iscritical in differentiating the gram-positive bacteria from the gram-negative bacteria. A prolonged
exposure to the decolorizing agent will remove all the stain from both types of bacteria. Some Gram-
positive bacteria may lose the stain easily and therefore appear as a mixture of Gram-positive and Gram-
negative bacteria (Gram-variable).
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Finally, a counterstain of basic fuchsin is applied to the smear to give decolorized gram-negative
bacteria a pink color. Some laboratories use safranin as a counterstain instead. Basic fuchsin stains many
Gram-negative bacteria more intensely than does safranin, making them easier to see. Some bacteria
which are poorly stained by safranin, such as Haemophilus spp., Legionella spp., and some anaerobic
bacteria, are readily stained by basic fuchsin, but not safranin. The polychromatic nature of the gram
stain enables determination of the size and shape of both Gram-negative and Gram-positive bacteria. If
desired, the slides can be permanently mounted and preserved for record keeping.
Besides Gram's stain, there are a wide range of other staining methods available. By using appropriate
dyes, different parts of the bacteria structures such as capsules, flagella, granules, and spores can be
stained. Staining techniques are widely used to visualize those components that are otherwise too
difficult to see under a light microscope. In addition, special stains can be used to visualize other
microorganisms not readily visualized by the Gram stain, such as mycobacteria, rickettsia, spirochetes,
and others. In addition, there are modifications of the Gram stain that allow morphologic analysis of
eukaryotic cells in clinical specimens.
AIM
To become familiar with
• The chemical and theoretical bases for differential staining procedures.
• The chemical basis of the gram stain.
• Performance of the procedure for differentiating between the two principal groups of
bacteria: gram-positive and gram-negative.
PRINCIPLE
Differential staining requires the use of at least three chemical reagents that are applied sequentially to
a heat-fixed smear. The first reagent is called the primary stain. Its function is to impart its color to all
cells. In order to establish a color contrast, the second reagent used is the decolorizing agent. Based onthe chemical composition of cellular components, the decolorizing agent may or may not remove the
primary stain from the entire cell or only from certain cell structures. The final reagent, the
counterstain, has a contrasting color to that of the primary stain. Following decolorization, if the
primary stain is not washed out, the counterstain cannot be absorbed and the cell or its components will
retain the color of the primary stain. If the primary stain is removed, the decolorized cellular
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components will accept and assume the contrasting color of the counterstain. In this way, cell types or
their structures can be distinguished from each other on the basis of the stain that is retained.
The most important differential stain used in bacteriology is the Gram stain, named after
Dr. Christian Gram. It divides bacterial cells into two major groups, gram-positive and gram-negative,
which makes it an essential tool for classification and differentiation of microorganisms. The Gram stain
uses four different reagents. Descriptions of these reagents and their mechanisms of action follow.
PRIMARY STAIN
Crystal Violet, this violet stain is used first and stains all cells purple.
MORDANT Gram’s Iodine serves as a substance that forms an insoluble complex by binding to the primary stain.
The resultant crystal violet-iodine (CV-I) complex serves to intensify the color of the stain, and all the
cells will appear purple-black at this point. In gram-positive cells only, this CV-I complex binds to the
magnesium-ribonucleic acid component of the cell wall. The resultant magnesium-ribonucleic acid-
crystal violet-iodine (Mg-RNA-CV-I) complex is more difficult to remove than the smaller CV-I
complex.
DECOLORIZING AGENT
Ethyl Alcohol, 95% serves a dual function as a lipid solvent and as a protein-dehydrating agent. Its
action is determined by the lipid concentration of the microbial cell walls. In gram-positive cells, the
low lipid concentration is important to retention of the Mg-RNA-CV-I complex. Therefore, the small
amount of lipid content is readily dissolved by the action of the alcohol, causing formation of minute
cell wall pores. These are then closed by alcohol’s dehydrating effect. As a consequence, the tightly
bound primary stain is difficult to remove, and the cells remain purple. In gram-negative cells, the high
lipid concentration found in outer layers of the cell wall is dissolved by the alcohol, creating large pores
in the cell wall that do not close appreciably on dehydration of cell wall proteins. This facilitates release
of the unbound CV-I complex, leaving these cells colorless or unstained.
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COUNTER STAIN
Safranin is the final reagent, used to stain red those cells that have been previously decolorized. Since
only gram-negative cells undergo decolorization, they may now absorb the counterstain. Gram-positive
cells retain the purple color of the primary stain.
The preparation of adequately stained smears requires that you bear in mind the
following precautions:
1. The most critical phase of the procedure is the decolorization step, which is based on the ease
with which the CV-I complex is released from the cell. Remember that over-decolorization will
result in loss of the primary stain, causing gram-positive organisms to appear gram-negative.
Under-decolorization, however, will not completely remove the CV-I complex, causing gram-
negative organisms to appear gram-positive. Strict adherence to all instructions will help remedy
part of the difficulty, but individual experience and practice are the keys to correct
decolorization.
2. It is imperative that slides be thoroughly washed under running tap water between applications
of the reagents. This removes excess reagent and prepares the slide for application of the
subsequent reagent.
3. The best gram stained preparations are made with fresh cultures, that is, not older than 24 hours.As cultures age, especially in the case of gram-positive cells, the organisms tend to lose their
ability to retain the primary stain and may appear to be gram-variable; that is, some cells will
appear purple, while others will appear red.
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DIAGRAM
GRAM STAINING
MATERIALS
CULTURES
24-hour nutrient agar slant cultures of microorganisms obtained from the soil sample(E.coli,Bacillus,
Proteus vulgaris,Pseudonomas).
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REAGENTS
Crystal violet, Gram’s iodine, 95%ethyl alcohol, and Safranin.
EQUIPMENTS
Bunsen burner, inoculating loop or needle, staining tray, glass slides, bibulous paper, lens paper and
microscope.
PROCEDURE
The steps are as follows;
1. Obtain four clean glass slides.
2. Using sterile technique, prepare a smear of each of the three organisms and on the remaining
slide prepare a smear consisting of a mixture of S.aureus and E.coli. Do this by placing a drop of
water on the slide and then transferring each organism separately to the drop of water on the
slide with a sterile, cooled loop. Mix and spread both organisms by means of a circular motion
of the inoculating loop.
3. Allow smears to air dry and then heat fix in the usual manner.
4. Flood smears with crystal violet and let stand for 1 minute.
5. Wash with tap water.
6. Flood smears with the gram’s iodine mordant and let stand for 1 minute.
7. Wash with tap water.
8. Decolorize with 95% ethyl alcohol. Caution: do not over decolorize. Add reagent drop by drop
until crystal violet fails to wash from smear.9. Wash with tap water.
10. Counterstain with Safranin for 45 seconds.
11. Wash with tap water.
12. Blot dry with bibulous paper and examine under oil immersion.
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OBSERVATION
1st slide appears red so gram negative bacteria.(E.coli).
2nd slide appears blue so gram positive bacteria(Bacillus).
3rd slide appears red so gram negative bacteria.(Proteus vulgaris)
4th slide appears red so gram negative bacteria.(Pseudomonas)
Typical Gram stain
GRAM POSITIVE GRAM NEGATIVE
RESULT
Both gram(+&-) bacteria are obtained in the soil sample.
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ENDOSPORE STAINING
THEORY
The endospore stain is a differential stain used to visualize bacterial endospores. Endospores are formed
by a few genera of bacteria, such as Bacillus. By forming spores, bacteria can survive in hostile
conditions. Spores are resistant to heat, dessication, chemicals, and radiation. Bacteria can form
endospores in approximately 6 to 8 hours after being exposed to adverse conditions. The normally-
growing cell that forms the endospore is called a vegetative cell. Spores are metabolically inactive and
dehydrated. They can remain viable for thousands of years. When spores are exposed to favorable
conditions, they can germinate into a vegetative cell within 90 minutes.
Endospores can form within different areas
of the vegetative cell. They can be central, subterminal, or terminal. Central endospores are located
within the middle of the vegetative cell. Terminal endospores are located at the end of the vegetative
cell. Subterminal endospores are located between the middle and the end of the cell.
Endospores can also be larger or smaller in
diameter than the vegetative cell. Those that are larger in diameter will produce an area of “swelling” in
the vegetative cell. These endospore characteristics are consistent within the spore-forming species and
can be used to identify the organism.
Because of their tough protein coats made of
keratin, spores are highly resistant to normal staining procedures. The primary stain in the endospore
stain procedure, malachite green, is driven into the cells with heat. Since malachite green is water-
soluble and does not adhere well to the cell, and since the vegetative cells have been disrupted by heat,
the malachite green rinses easily from the vegetative cells, allowing them to readily take up the
counterstain.
AIM - To identify the endospore forming bacteria in the soil sample.
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REQUIRMENTS -
Malachite green, safarine, staining tray, glass slide,pure cultures. (E.coli,Bacillus, Proteus
vulgaris,Pseudonomas).
PROCEDURE
1. Make smears of the 5 pure samples on the slide.
2. Steam for 5 min and add malachite green time to time.
3. Wash under running water.
4. Blot dry the slides
5. Add safrenin to it keep for 10 min
6. Wash it.
OBSERVATION
If colour comes to green then it is endospore former otherwise if the colour comes non green then it is
non endospore former.
1ST slide is not green therefore non endospore former bacteria.(E.coli)
2nd slide is green therefore endospore former bacteria.(Bacillus)
3rd slide is not green therefore non endospore former bacteria.(Proteus vulgaris)
4th slide is not green therefore non endospore former bacteria.(Pseudomonas)
DIAGRAM
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: ENDOSPORE FORMING BACTERIA
RESULT
Both endospore former and non former bacteria obtained fro the soil sample
.
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SCREENING OF MICROORGANISMS FOR
INDUSTERIAL PURPOSE
AIM : Screening of proteases (caseinase) producing bacteria.
THEORY
Proteases are the single class of enzymes, which occupy a pivotal position with respect to
their applications in both physiological and commercial fields.
They perform both degradative and synthetic functions. Proteolytic enzymes catalyze the
cleavage of peptide bonds in other proteins. Advances in analytical technique have
demonstrated that proteases conduct highly specific and selective modifications of
proteins.
Proteases are classified on the basis if three major criteria: (1) Type of reaction catalyzed
(2) Chemical nature of the catalytic site and (3) Evolutionary relationship with reference
to structure.
Proteases are grossly subdivided into two major groups’ i.e., exopeptides and
endopeptides, depending on their site of action.
Based on the functional group present at the site active site, proteases are further classified
into 4 prominent groups i.e. serine proteases, cysteine proteases, aspartic proteases and
metallo proteases.
Proteases are also divided into acid, neutral and alkaline proteases on the basis of pH
range in which their activity is optimum.
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Proteases occur ubiquitously in a wide diversity of sources such as plants, animals and
microorganisms. Microbes are the attractive sources of proteases and have gained much
popularity than any other sources because of their broad biochemical diversity.
The inability of the plant and animal proteases to meet current world demands has lead to
an increased interest in microbial proteases.
Microbial enzymes have two advantages over the animal and plant enzyme. Firstly, they
are economical and can be produced on a large scale within the limited space and time. It
can be easily extracted and purified.
Secondly, there is a technical advantage in producing enzymes via using micro organisms
as (1) they are capable of producing wide variety of enzymes (2) they show geneticflexibility that is why they can be genetically manipulated to increase the yield of
enzymes and they have a short generation time.
Proteases execute a large variety of functions, extending from the cellular level to the
organ and organism level. Their involvement in the life cycle of disease organisms has
lead them to become a potential target for developing therapeutic agents against fatal
disease such as cancer and AIDS.
Proteases have a long history of applications in different industries viz, detergents, food-
brewing, meat tenderization, baking, manufacture of Soya products, debittering of protein
hydrolysis’s , synthesis of aspartame, dairy, leather, silk and for recovery of silver from
used x-ray films.
Besides their industrial and medicinal applications, proteases play an important role in
basic research. Their selective peptide bond cleavage is used in the study of sequencing of
proteins.
A wide range of microorganisms including bacteria, yeast and also mammalian tissues
produces alkaline proteases.
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CASEIN
Casein (from Latin caseus "cheese") is the predominant phosphoprotein.that account for
nearly 80% of proteins in milk and cheese. Milk-clotting proteases act on the soluble portion of the caseins, K-Casein, thus originating an unstable micellar state that results in
clot formation. When coagulated with rennet, casein is sometimes called paracasein.
Chymosin (EC 3.4.23.4) is an aspartic protease that specifically hydrolyzes the peptide
bond in Phe105-Met106 of κ-casein and is considered to be the most efficient protease
for the cheese-making industry.British terminology, on the other hand, uses the term
caseinogen for the uncoagulated protein and casein for the coagulated protein.
As it exists in milk, it is a salt of calcium. Casein is not coagulated by heat. It is
precipitated by acids and by rennet enzymes, a proteolytic enzyme typically obtainedfrom the stomachs of calves.
The enzyme trypsin can hydrolyze off a phosphate-containing peptone.
Casein consists of a fairly high number of proline peptides, which do not interact. There
are also no disulfide bridges. As a result, it has relatively little secondary structure or
tertiary structure. Because of this, it cannot denature. It is relatively hydrophobic, making
it poorly soluble in water. It is found in milk as a suspension of particles called casein
micelles which show some resemblance with surfactant-type micellae in a sense that the
hydrophilic parts reside at the surface.
The caseins in the micelles are held together by calcium ions and hydrophobic
interactions. There are several models that account for the special conformation of casein
in the micelles. One of them proposes that the micellar nucleus is formed by several
submicelles, the periphery consisting of microvellosities of κ-casein. Another model
suggests that the nucleus is formed by casein-interlinked fibrils
Finally, the most recent model proposes a double link among the caseins for gelling to
take place. All 3 models consider micelles as colloidal particles formed by casein
aggregates wrapped up in soluble κ-casein molecules.
The isoelectric point of casein is 4.6. The purified protein is water insoluble.
While it is also insoluble in neutral salt solutions, it is readily dispersible in dilute alkalis
and in salt solutions such as sodium oxalate and sodium acetate.
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PRINCIPLE:
It is based on the principle that some microorganisms have the ability to degrade the protein, casein
by producing proteolytic exoenzymes, proteinase or caseinase, which breaks the peptide bond CO-NH
into free amino acids.
REQUIRMENTS:
Slant culture of test organism(E.COLI)
Skimmed milk agar. or casein media
1. Skim milk powder 10g
2. Peptone 0.5g
3. Agar 1.5g
4. ph 7.2(adjust ph by ph meter)
5. Distilled water 100ml
Petri plate
Inoculating loop
PROCEDURE:
The autoclaved skimmed milk medium was poured into sterile plate and allowed to solidify
.Upon solidification of the medium single round streak inoculation was done from each isolate at the
two sides of the plate. The plate was incubated at 30°C for 24-48 hours in an inverted position.
After incubation the plate was observed for any clear zones around the growth of the organisms.
Mass production of the enzyme can be done either by submerged fermentation or solid substrate
fermentation. In submerged fermentation, the organism was cultivated in liquid media in the flasks for the enzyme production whereas in the solid substrate fermentation, the culture was inoculated across the
surface of production medium and the culture remains on the surface through out the fermentation.
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OBSERVATION:
A clear zones around the growth of the organisms is observed.
DIAGRAM:
CASEIN DEGRADATION
RESULT:
Screening of proteases producing microorganism done.
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AIM : Screening of Amylase producing bacteria by starch hydrolysis.
THEORY
The ability to degrade starch is used as a criterion for the determination of amylase production
by a microbe. In the laboratory it is tested by performing the starch test to determine the absence or
presence of starch in the medium by using iodine vapor as an indicator. Starch in the presence of iodine
produces a dark blue coloration of the medium around the colony.
PRINCIPLE:
The extracellular enzyme alpha amylase catalyzes the breakdown of starch to maltose. The smaller
maltose molecules can enter the cell to be used for energy. Iodine interacts with starch and makes it dark
blue. If starch has been removed from a culture medium by the action of the bacterial enzyme no blue
color appears in the presence of iodine. If iodine stains the starch medium blue in the presence of
growing bacterial colonies then no amylase is produced by that species
REQUIRMENTS
Starch agar media
1. Starch 2g
2. Peptone 0.5g
3. Beef extract 0.3g
4. Agar 1.5g
5. dDstilled water 100 ml
Petriplates
Previously cultured media(bacillus culture)
Inoculating loop
PROCEDURE
The starch agar medium was melted, cooled to 450C and poured into the sterile Petri dish.
Allowed it to solidify,
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Using sterile techniques a single streak inoculation of Bacillus subtilis was made at the center of
the Petri plate.
The Petri plates were incubated for 72 hours at room temperature.
A Luxurious growth of Bacillus subtilis was seen along the streak.
The plates were exposed to Iodine vapors.or iodinr added to them.
OBSERVATION
The zone of clearing surrounding Bacillus indicate that it was able to hydrolyze starch. Due to which a
clear sharp boundry of transparent type is developed.
DIAGRAM
STARCH DEGRADATION SHOWING AMYLASE PRODUCTION
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CLOSE UP
RESULT:
Screening of Amylase producing bacteria by starch hydrolysis done.
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REFERENCES
1. Madigan M, Martinko J (editors) (2006). Brock Biology of Microorganisms,11th ed., Prentice Hall. ISBN 0-13-144329-1.
2. Rice G (2007-03-27). Are Viruses Alive?. Retrieved on 2007-07-23.
3. Amann RI, Ludwig W, Schleifer KH (1995). "Phylogenetic identification and insitu detection of individual microbial cells without cultivation". Microbiol.Rev. 59: 143-169.
4. Varro On Agriculture 1,xii Loeb
5. Ibrahim B. Syed, Ph.D. (2002). "Islamic Medicine: 1000 years ahead of itstimes", Journal of the Islamic Medical Association 2, p. 2-9.
6. David W. Tschanz, MSPH, PhD (August 2003). "Arab Roots of EuropeanMedicine", Heart Views 4 (2).
7. Gest H (2005). "The remarkable vision of Robert Hooke (1635-1703): firstobserver of the microbial world". Perspect. Biol. Med. 48 (2): 266-72.
8. doi :10.1353/pbm.2005.0053. PMID 15834198.
9. Drews G (1999). "Ferdinand Cohn, a Founder of Modern Microbiology". ASMNews 65 (8).
10.Ryan KJ, Ray CG (editors) (2004). Sherris Medical Microbiology , 4th ed.,McGraw Hill. ISBN 0-8385-8529-9.