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What is covalent bonding?
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In hydrogen bonding, the individual bonds are very strong.
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The sub-unit of a polysaccharide is a [blank_start]monosaccharide[blank_end]. Two of these together form a disaccharide.
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monosaccharide
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mononucleotide
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disaccharide
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glucose
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Formation of polypeptides and polysaccharides are ____________ reactions.
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condensation
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hydrolysis
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magic
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A molar solution is a solution that contains [blank_start]1 mol of solute in a litre of solution[blank_end]
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[blank_start]Monomers[blank_end] join together to make [blank_start]polymers[blank_end].
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Monomers
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Polymers
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Nucleotides
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polymers
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monomers
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glucose
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Monosaccharides are...
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The test for reducing sugars involves adding hydrochloric acid
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A reducing sugar is a sugar that can reduce another substance by [blank_start]donating its electrons[blank_end]
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To test for reducing and non-reducing sugars we use...
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Tollen's reagent
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Benedict's reagent
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Starch
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Iodine
Frage 11
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What are the results of the Benedict's test for reducing sugars?
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Turns red for a high concentration
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Stays blue for no reducing sugars
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Turns green for a high concentration
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Turns yellow/orange for a medium concentration
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Turns purple for a low concentration
Frage 12
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Glucose plus [blank_start]glucose[blank_end] forms maltose.
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Glucose plus [blank_start]fructose[blank_end] forms sucrose.
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fructose
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glucose
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galactose
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Glucose plus [blank_start]galactose[blank_end] forms lactose.
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fructose
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galactose
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sucrose
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What is this molecule?
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What is this molecule?
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How does the Benedict's test for non-reducing sugars differ to that of reducing sugars? (tick all appropriate)
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The colour changes are different
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You have to add hydrochloric acid after the first round of heating
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You add nitrogen sulphide to neutralise the acid
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You add sodium hydroxide to neutralise the acid
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There is a temperature change after you add the iodine
Frage 18
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Polysaccharides are insoluble
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The test for starch uses [blank_start]iodine[blank_end]. If starch is present it will turn from [blank_start]orange[blank_end] to [blank_start]black[blank_end].
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iodine
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Tollen's reagent
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orange
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red
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blue
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silver
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black
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purple
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Starch is made of alpha glucose.
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Tick the correct answers.
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Cellulose is found in plants
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Cellulose is made of alpha glucose
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Glycogen is found in bacteria
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Glycogen is made of alpha glucose
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Starch is linked by glycosidic bonds
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Starch is a straight molecule
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Glycogen is short coils with lots of branches
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Cellulose is branched
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Cellulose has hydrogen bonds that form cross-linkages
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Lipids are insoluble in [blank_start]water[blank_end] but soluble in [blank_start]organic solvents[blank_end]
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What are some roles of lipids?
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What is this molecule?
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The fatty acids in triglycerides are unsaturated.
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Structure and functions of triglycerides:
The high ratio of carbon-hydrogen bonds to carbon atoms means they are a good [blank_start]source of energy[blank_end].
The low mass to energy ratio means they are good [blank_start]storage molecules[blank_end].
The large and insoluble molecules are [blank_start]good storage molecules[blank_end] and don't affect the [blank_start]water potential[blank_end] of the cells.
The high ration of hydrogen to oxygen atoms mean they are a good [blank_start]source of water[blank_end].
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source of energy
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storage molecules
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good storage molecules
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water potential
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source of water
Frage 28
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What is this molecule?
Frage 29
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Phospholipids have...
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A hydrophilic head
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A hydrophobic head
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A hydrophilic tail
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A hydrophobic tail
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Structure and function of phospholipids:
The hydrophilic heads and hydrophobic tails form a [blank_start]bilayer[blank_end] in [blank_start]aqueous[blank_end] environments.
The [blank_start]hydrophilic[blank_end] heads help hold the surface of the cell-surface membrane.
They can form [blank_start]glycolipids[blank_end] with carbohydrates which are important for cell recognition.
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bilayer
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aqueous
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gaseous
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hydrophilic
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glycolipids
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emulsions
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Test for lipids:
1. Add 2cm^3 of your sample and 5cm^3 of [blank_start]ethanol[blank_end] to a test tube
2. Shake the tube to dissolve any [blank_start]lipids[blank_end] in the sample
3. Add 5cm^3 of [blank_start]water[blank_end] and shake gently
4. If lipids are present then the solution will turn [blank_start]cloudy-white[blank_end]
Antworten
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ethanol
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iodine
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lipids
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glucose
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water
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Benedict's reagent
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cloudy-white
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yellow
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blue
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black
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Amino acids are the basic [blank_start]monomer[blank_end] units for proteins and the polymer is called a [blank_start]polypeptide[blank_end].
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monomer
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polymer
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sugar
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polynucleotide
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polypeptide
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polysaccharide
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Amino acids provide indirect evidence for...
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Evolution (the same 40 are in everything)
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Meiosis (each is split in two for gametes)
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Evolution (the same 20 are in everything)
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Mitosis (the same ones are in the daughter cells)
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Label this amino acid structure
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R group
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Nitrogen
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Amino group
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Phosphate
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Carboxyl group
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Carbohydrate
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Hydrochloric acid
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Hydrogen
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Central carbon atom
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Central carbon ion
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The process of joining many amino acid monomers together is called polymerisation.
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The primary structure of a protein is formed by the specific sequence of [blank_start]amino acids[blank_end]. The primary structure determines its [blank_start]shape[blank_end] and therefore function so changing just a single amino acid in the chain could potentially change the way the whole protein works.
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The [blank_start]secondary[blank_end] structure of a protein is the long polypeptide chain being twisted into a [blank_start]3D[blank_end] shape. This is caused by the [blank_start]hydrogen[blank_end] bonds that form between the H from the [blank_start]positive[blank_end] NH group of one and the O of another's [blank_start]negative[blank_end] C=O.
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secondary
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tertiary
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2D
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3D
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hydrogen
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disulfide
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positive
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negative
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positive
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negative
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The tertiary structure of the protein is formed by the secondary structure being further coiled and twisted into a more [blank_start]complex[blank_end] and recognisable shape. This shape is maintained by three types of bonds: hydrogen bonds, [blank_start]ionic[blank_end] bonds and disulfide bridges. The [blank_start]hydrogen[blank_end] bonds are numerous but easily broken. The ionic bonds are stronger than the hydrogen bonds however they are easily broken by a change in [blank_start]pH[blank_end]. The disulfide bridges are the [blank_start]strongest[blank_end] out of the three.
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complex
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hydrogen
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pH
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temperature
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pressure
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strongest
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weakest
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ionic
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The [blank_start]quaternary[blank_end] structure is the most complex and consists of many individual polypeptide chain linked in various ways. Some of these molecules have non-protein ([blank_start]prosthetic[blank_end]) groups associated with them e.g. the [blank_start]iron[blank_end] containing haem group in haemoglobin.
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quaternary
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tertiary
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secondary
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fake
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prosthetic
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pseudo
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iron
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nitrogen
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calcium
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magnesium
Frage 40
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What is the test for proteins called?
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Tollen's
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Sterilisation
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Biuret
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Benedict's
Frage 41
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What are the steps in the test for proteins?
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1. Place your sample and an equal volume of sodium hydroxide in a test tube
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1. Place your sample and an equal volume of sodium disulphate in a test tube
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!. Place your sample and an equal volume of hydrochloric acid in a test tube
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2. Add a few drops of high concentration copper sulphate and mix gently
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2. Add a few drops of very dilute copper sulphate and mix gently
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3. If it goes red there are peptide bonds and therefore proteins present but stays blue in their absence
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3. If it goes purple there are peptide bonds and therefore proteins present but stays blue in their absence
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3. If it goes green there are peptide bonds and therefore proteins present but stays blue in their absence
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Enzymes are globular proteins that act as [blank_start]catalysts[blank_end]. They do this by lowering the [blank_start]activation energy[blank_end] of a reaction by providing an alternative pathway for the reaction without being [blank_start]used up[blank_end] themselves.
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catalysts
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activation energy
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used up
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The functional region of an enzyme is called the...
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substrate
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active site
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complex
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The molecule upon which the enzyme acts is called the...
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substrate
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active site
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protein
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Scientists used to use the [blank_start]lock and key[blank_end] model to explain how enzymes work but this is now out-dated. Instead, we use the [blank_start]induced-fit[blank_end] model. It suggests that the enzyme's active site changes shape when in close proximity to the [blank_start]substrate[blank_end] as a result of the [blank_start]charges[blank_end] in each molecule. The active site [blank_start]moulds[blank_end] itself around the substrate to form an [blank_start]enzyme-substrate complex[blank_end] which distorts bonds in the substrate to lower the [blank_start]activation[blank_end] energy.
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lock and key
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induced-fit
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substrate
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charges
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moulds
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enzyme-substrate complex
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activation
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For an enzyme to work, it must...
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Come into contact with the substrate
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Be diluted in solution
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Have the correct orientation so the active site and substrate collide
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Have a complementary active site to the substrate
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Be at body temperature (37°C)
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The two changes most frequently measured to measure the rate of enzyme-catalysed reactions are...
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Measuring rate of change on a graph involves drawing a tangent to the curve and then working out the change in x divided by the change in y.
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Label this graph of the effects of temperature on enzyme activity
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Optimum temperature
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Temp too high, enzymes start to denature
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As temp increases, kinetic energy does
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Temp too low, not enough energy to work
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No enzymes left, no activity
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Label this graph of the effects of pH on enzyme activity
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Label this graph of the effects of enzyme concentration on enzyme activity
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Too few enzymes for amount of substrate
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All substrate has an active site
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Already enough active sites for sub.
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Temperature too high
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Not enough kinetic energy
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Optimum pH
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Label this graph of the effects of substrate concentration on enzyme activity
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Not enough sub. to fill all active sites
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Max rate, all sub in an active site
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All active sites already occupied
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Temperature too high
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Optimum pH
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Not enough kinetic energy
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[blank_start]Competitive[blank_end] inhibitors interfere with the functioning of an enzyme by binding to the active site and getting in the way of the substrate. [blank_start]Non-competitive[blank_end] inhibitors interfere with the functioning of an enzyme by binding to it in a place other than the active site, changing its shape so the active site is no longer [blank_start]complementary[blank_end] to the substrate.
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Competitive
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Non-competitive
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complementary
Frage 54
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Competitive
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Non-competitive
Frage 55
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Competitive
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Non-competitive