biotechnology - PowerPoint PPT Presentation

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biotechnology

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Title: biotechnology


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BIOTECHNOLOGY
  • (PRODUCTS AND TECHNIQUES OF PRODUCTION)

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  • Biotechnology is defined by the US government as
    any technique that uses living organisms (or
    parts of organisms) to make or modify products,
    to improve plants and animals or to develop
    microorganisms for specific uses.
  • Biotechnology is the use of living systems and
    organisms to develop or make products.

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  • ?any technological application that uses
    biological systems, living organisms or
    derivatives thereof, to make or modify products
    or processes for specific use
  • ?For thousands of years, humankind has used
    biotechnology in agriculture, food production,
    and medicine.

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  • BRANCHES OF BIOTECHNOLOGY
  • ?A series of derived terms have been coined to
    identify several branches of biotechnology

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  • ?Bioinformatics - is an interdisciplinary field
    which addresses biological problems using
    computational techniques, and makes the rapid
    organization as well as analysis of biological
    data possible.

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  • ?Blue biotechnology - is a term that has been
    used to describe the marine and aquatic
    applications of biotechnology, but its use is
    relatively rare.
  • ?White biotechnology-also known as industrial
    biotechnology, is biotechnology applied to
    industrial processes.

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  • ?Green biotechnology - is biotechnology applied
    to agricultural processes.
  • ?Red biotechnology is applied to medical
    processes.

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IMPORTANCE OF BIOTECHNOLOGY ?A wide
variety of microorganisms are now being employed
as tools in biotechnology to produce useful
products or services.
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  • ?Raw materials can be converted to useful
    finished products.
  • ?Biotechnologically produced organic acids like
    citric acid, acetic acid, gluconic acid, D-Lactic
    acid, fumaric acid, etc. also has very high
    market value.
  • ?Biotechnology is widely used in pharmacy to
    create more efficient and less expensive drugs.

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TECHNIQUES USED IN THE PRODUCTION OF
BIOTECHNOLOGICS
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RECOMBINANT DNA (rDNA)
  • joining together of DNA molecules from two
    different species that are inserted into a host
    organism to produce new genetic combinations that
    are of value to science, medicine, agriculture,
    and industry. Since the focus of all genetics is
    the gene, the fundamental goal of laboratory
    geneticists is to isolate, characterize, and
    manipulate genes. Although it is relatively easy
    to isolate a sample of DNA from a collection of
    cells, finding a specific gene within this DNA
    sample can be compared to finding a needle in a
    haystack. Consider the fact that each human cell
    contains approximately 2 metres (6 feet) of DNA.

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  • Therefore, a small tissue sample will contain
    many kilometres of DNA. However, recombinant DNA
    technology has made it possible to isolate one
    gene or any other segment of DNA, enabling
    researchers to determine its nucleotide sequence,
    study its transcripts, mutate it in highly
    specific ways, and reinsert the modified sequence
    into a living organism.

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MONOCLONAL ANTIBODIES
  • antibody produced artificially by a genetic
    engineering technique. Production of monoclonal
    antibodies was one of the most important
    techniques of biotechnology to emerge during the
    last quarter of the 20th century.

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  • When activated by an antigen, a circulating B
    cell multiplies to form a clone of plasma cells,
    each secreting identical immunoglobulin
    molecules. It is such immunoglobulinsderived
    from the descendants of a single B cellthat are
    called monoclonal antibodies.

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  • The antibody response to a natural infection or
    an active immunization, however, is polyclonal.
    In other words, it involves many B cells, each of
    which recognizes a different antigenic
    determinant (epitope) of the immunizing antigen
    and secretes a different immunoglobulin.

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  • Thus the blood serum of an immunized person or
    animal normally contains a mixture of antibodies,
    all capable of combining with the same antigen
    but with different epitopes that appear on the
    surface of the antigen.

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  • Furthermore, even antibodies that bind to the
    same epitope often have different abilities to
    bind to that epitope. This makes isolating an
    appreciable quantity of a particular monoclonal
    antibody from the polyclonal mixture extremely
    difficult.

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POLYMERASE CHAIN REACTION (PCR)
  • a technique used to make numerous copies of a
    specific segment of DNA quickly and accurately.
    The polymerase chain reaction enables
    investigators to obtain the large quantities of
    DNA that are required for various experiments and
    procedures in molecular biology, forensic
    analysis, evolutionary biology, and medical
    diagnostics.

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  • The PCR technique is based on the natural
    processes a cell uses to replicate a new DNA
    strand. Only a few biological ingredients are
    needed for PCR. The integral component is
    the template DNAi.e., the DNA that contains the
    region to be copied, such as a gene. As little as
    one DNA molecule can serve as a template. The
    only information needed for this fragment to be
    replicated is the sequence of two short regions
    of nucleotides (the subunits of DNA) at either
    end of the region of interest.

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These two short template sequences must
be known so that two primersshort stretches of
nucleotides that correspond to the template
sequencescan be synthesized. The primers bind,
or anneal, to the template at their complementary
sites and serve as the starting point for
copying. DNA synthesis at one primer is directed
toward the other, resulting in replication of the
desired intervening sequence.
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  • Also needed are free nucleotides used to build
    the new DNA strands and a DNA polymerase,
    anenzyme that does the building by sequentially
    adding on free nucleotides according to the
    instructions of the template.
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