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Summary OCR A level biology cell structure notes made from the specification

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My OCR A-Level Biology Cell Structure A3 summary sheet is just a clear, no-nonsense page with everything you actually need for the OCR spec. It covers organelles, prokaryotes vs eukaryotes, microscopy, and key definitions in a simple layout that’s easy to scan. No long paragraphs, no waffle — just key terms, and the points examiners look for. Perfect for quick revision the night before a test or when you need everything in one place.

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​Cell structure​
​ )​
a ​ )​
b c​ )​
​Light microscopes:​ ​calibrating eyepiece graticules and stage micrometers​ ​How to stain a sample​
​●​ ​Light is shone up the base, through the sample, up through the​ ​1.​ ​Use a pipette to place a small drop of water onto the centre of the​
​objective lens into our eye​ ​glass slide​
​●​ ​The specimen used has to be thin so light can pass through it​ ​2.​ ​Use a pair of forceps (tweezers) to place a thin section of the​
​●​ ​The specimen can be alive but sometimes the light causes heat​ ​specimen onto the drop of water.​
​which can damage the organism​ ​3.​ ​The specimen should be thin enough to allow light to pass through.​
​●​ ​Used to look at whole cells and tissues, you cannot see organelle​ ​4.​ ​Add a few drops of stain to the specimen.​
​detail in a light microscope​ ​●​ W ​ hen viewing a specimen you can use an eyepiece graticule to​ ​5.​ ​Slowly add a cover slip on the specimen​
​measure its width and length​
​Electron microscopes:​ ​ ry mounts​​- the specimen is placed directly onto the slide and covered​
D
​●​ ​Eyepiece graticule is a small scale placed within the eyepiece​
​●​ ​Use electrons to form an image​ ​with a cover slip​
​●​ ​Since electrons have a shorter wavelength than light, they have a​ ​●​ ​The scale divisions will represent different real world distances​
​depending on the magnification of the objective lens. This means​ ​c) staining:​
​better resolution than light microscopes​
​Coloured staining binds to chemicals on or in the specimen which allows​
​●​ ​However, they’re more expensive than light microscopes and only​ ​the graticule must be calibrated for each objective lens​
​the specimen to become visible, to see certain organelles and it improves​
​produce black and white images (computers can add colour to​ ​●​ ​A stage micrometre is used to calibrate the graticule​ ​contrast​
​these images)​ ​●​ ​Stage micrometre is a glass slide with a scale measured in​ ​Some stains bind to specific cell structures - eosin stains cytoplasm pink​
​●​ ​These microscopes require complex preparation of specimens so​ ​micrometres​ ​and sudan stains membranes and other lipids black​
​they are more likely to create artefacts.​
​Artefacts = visible details that aren't part of the specimen being observed,​ ​The graticule is calibrated as follows:​
​Differential staining is using more than 1 chemical stain​
​like air bubbles or finger prints​ ​ .​ F
1 ​ ix the stage micrometer into place on the stage.​
​2.​ ​Look through the eyepiece to line up the micrometer and the​
​Transmission electron microscope:​
​graticule.​ i​)​
​●​ ​They use electromagnets to transmit a beam of electrons through a​
​3.​ ​Count the number of graticule divisions that fit into one micrometer​ ​Secretion of proteins (enzymes or hormone)​
​specimen so you can see details inside the specimen​
​division.​ ​●​ ​Normally to produce a protein such as an enzyme or a protein​
​●​ ​The denser parts absorb more electrons so appear darker in the​
​image formed​ ​4.​ ​Use the formula below to calculate the size of each graticule​
​1.​ T ​ he nucleus is producing mRNA which leaves the​​nucleus​​through​
​●​ ​specimens have to be thin enough to allow the electrons to pass​ ​division at that magnification:​ ​the​​nuclear pore​
​through​ ​ raticle division = size of 1 micrometer division / number of graticule​
G ​2.​ ​The mRNA will attach to a​​ribosome​​- the ribosome may be​
​●​ ​The specimen has to be viewed in a vacuum so only non living or​
​divisions​ ​attached to the RER or free in the cytoplasm​
​dead organisms can be observed​
​3.​ ​The protein is made via protein synthesis in the ribosome​
​●​ ​Used to look at organelle detail​
​4.​ ​The protein is transported via a​​vesicle​​to the​​golgi apparatus​
​●​ ​TEM images can appear differently if the cell/organelle has been​ ​Steps for viewing a microscope slide​ ​5.​ ​This is where the protein is modified and packaged, for example it​
​cut along different planes/angles or it's become an artifact so it's​ ​1.​ ​Clip the prepared slide onto the stage​ ​could be combined with a carbohydrate to form a glycoprotein​
​been damaged and doesn't look how it's supposed to.​
​2.​ ​Select the objective lens with the lowest power​ ​6.​ ​The protein is then packaged into a​​vesicle​​again​
​3.​ ​Use the coarse focus to move the stage just below the lens​ ​7.​ ​The vesicle is moved to the​​cell surface membrane​​of the cell​
​Scanning electron microscope​
​4.​ ​Look through the eyepiece and use the coarse focus to move the​ ​where exocytosis will occur​
​●​ ​Used to look at the cell surface detail or the organelle details​
​●​ ​They scan a beam of electrons across the surface of a specimen -​ ​stage until the image is roughly in focus​
​ he mitochondria produces ATP which helps the cytoskeleton contract and​
T
​the reflected electrons are used to form an image​ ​5.​ ​Use the fine focus to make the image clearer​ ​move the vesicle from the golgi body to the cell surface membrane to allow​
​●​ ​They produce 3D images​ ​6.​ ​Is a higher magnification is needed swap the objective lens and​ ​exocytosis to occur.​
​●​ ​Similarly to TEMs, they can only view non living or dead specimens​ ​refocus​
​but SEMs can be used on thicker specimens​

​ )​
d ​e) and f)​ ​k) the difference between eukaryotic and prokaryotic cells​
​biological drawings​
​ agnification = the number of times larger the image is in comparison to​
M ​●​ E ​ ukaryotic cells have membrane bound organelles and a distinct​
​Biological drawings should not:​ ​the object​ ​nucleus whereas prokaryotes don’t.​
​●​ ​Include shading or colouring​ ​Resolution = the ability to distinguish between very small structures that​ ​●​ ​Ribosomes in a eukaryotic cell is 80s whereas in prokaryotes its​
​●​ ​Include arrow heads for labels​ ​are close together, in detail​ ​70s​
​●​ ​Include overlapping lies​ ​●​ ​Eukaryotic organisms have linear DNA whereas prokaryotic​
​Biological drawings should:​ ​Magnification = image size/actual size​ ​organisms have circular DNA​
​●​ ​Include a title​ ​●​ ​The cell wall in eukaryotes is made of cellulose and in prokaryotes​
​●​ ​State the magnification / scale​ ​ ight microscope:​
L ​its made of murein/ peptidoglycan​
​●​ ​Be drawn with a sharp pencil​ ​Resolution = 0.2 micrometers Magnification = x 1,500​ ​Difference between animal and plant cells​
​●​ ​Include smooth, continuous lines​ ​TEM​ ​●​ ​Plant cells have a vacuole, cell walls and chloroplasts but animal​
​●​ ​Include labels​ ​Resolution = 0.5 nanometers Magnification = x1,500,000​ ​cells dnt​
​●​ ​Include accurate sizes of observable structures​ ​SEM​
​Resolution = 5 nanometers Magnification = x1,500,000​

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Subido en
1 de marzo de 2026
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Escrito en
2025/2026
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