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Summary A Level Biology Cell Structure and Microscopes Notes

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This pack of notes contains detailed information about scanning, transmission and light microscopes, mitosis and the cell cycle, cancer and animal and plant organelles. These notes helped me achieve an A* in my term exams and an A in my A level exams.

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CELL STRUCTURE
(3.1-3.8)

3.1 Methods of studying cells



Microscopy

What are microscopes? Instruments that produce a magnified image of an
object.

Microscope lenses work more effectively if the convex glass lenses are used in
pairs in a compound light microscope.

● Light microscopes - the relatively long wavelength of light rays means
that a light microscope can only distinguish between two objects if they
are 0.2μm, or further apart.



This limitation can be overcome by using beams of ELECTRONS rather than
beams of light.

● Electron microscopes - with their shorter wavelengths, a beam of
electrons in the electron microscope can distinguish between two
objects only 0.1nm apart.




Magnification

The material that is put under a microscope is referred to as the object. The
appearance of this material when viewed under the microscope is referred to
as the image.

,Magnification: the magnification of an object is how many times bigger the
image is when compared to the size of the real object.

Magnification = size of image/size of real object
Size of real object = size of image/magnification



When calculating magnification, make sure that the units of length are the
same for both the object and the image!



Resolution

Resolution/resolving power: the resolution or resolving power of a microscope
is the minimum distance apart that two objects can be in order for them to
appear as separate items.

● The resolving power depends on the wavelength or form of radiation
used.
● A light microscope has a resolution of about 0.2μm (any two objects that
are 0.2μm or more apart will be seen separately but if they are closer
than this, they will appear as a single item).

● Greater resolution means greater CLARITY.

● The image produced with a high resolution is clearer and more PRECISE.

● Increasing magnification increases the size of the image but doesn’t
always increase the resolution.

● Every microscope has a limit of resolution. Up to this point, increasing
the magnification will reveal more detail, but beyond this point
increasing the magnification will not do this.

● The object will still appear larger but more blurred instead!

, Cell fractionation

To study the structure and function of the various organelles that make up
cells, it is necessary to obtain large numbers of ISOLATED organelles.

Cell fractionation: the process where cells are broken up and the different
organelles they contain are separated out.

Process of cell fractionation:

1. Homogenation
2. Ultracentrifugation



BEFORE cell fractionation begins, the tissue is placed in a cold, buffered
solution which has the same water potential as the tissue. The solution is:

● Cold - to reduce enzyme activity that might break down the organelles.

● Buffered - so that the pH does not fluctuate. Any change in pH could
affect the functioning of enzymes and also alter the structure of the
organelles.

● Of the same water potential as the tissue - to prevent the organelles
from shrinking or bursting due to osmotic loss or gain of water.



Stages of cell fractionation:

1. HOMOGENATION

- The cells are broken up inside a homogeniser (blender)

, - The various organelles from the cell are released.
- The resulting fluid is called the homogenate.
- The homogenate is filtered to remove any complete cells and large
pieces of debris.



2. ULTRACENTRIFUGATION

Ultracentrifugation: the process by which the fragments in the filtered
homogenate are separated in a machine called a centrifuge.

The centrifuge spins tubes of homogenate at very high speeds in order to
create a centrifugal force.

For animal cells, the process goes like this:

○ The tube of filtrate is placed in the centrifuge and spun at a slow speed.

○ The heaviest organelles i.e. the nuclei are forced to the bottom of the
tube where they form a thin sediment or pellet.



○ The fluid at the top, supernatant, is then removed leaving only the
sediment of nuclei.

○ The supernatant is transferred to another tube and spun in the
centrifuge at a FASTER speed than before.



○ The next heaviest organelles i.e. the mitochondria are forced to the
bottom of the tube.



○ The process is continued in this way so that, at each increase in speed,
the next heaviest organelle is sedimented and separated out.
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