BIOL 305L Laboratory Two



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Please print Full name clearly: Introduction BIOL 305L Laboratory Two Osmosis, because it is different in plants! Osmosis is the movement of solvent molecules through a selectively permeable membrane into a region of higher solute concentration, aiming to equalize the solute concentrations on the two sides. The term osmosis may also be used to describe a physical process in which any solvent moves, without input of energy, across a semi-permeable membrane (permeable to the solvent, but not the solute) separating two solutions of different concentrations. Although osmosis does not require input of energy, it does use kinetic energy and can be made to do work. The first documented observation of osmosis was made by Jean-Antoine Nollet (19th November 1700 25th April 1770) in 1748, who was a French clergyman and physicist. Osmosis is essential in biological systems, as biological membranes are semipermeable. In general, these membranes are impermeable to large and polar molecules, such as ions, proteins, and polysaccharides, while being permeable to nonpolar and/or hydrophobic molecules like lipids as well as to small molecules like oxygen, carbon dioxide, nitrogen, nitric oxide. Tonicity is the osmolarity of a solution--the amount of solute in a solution. A Solute is any dissolved substance in a solution, such as sugars and salts. The term Tonicity is commonly used when describing the response of cells immersed in an external solution. Like osmotic pressure, tonicity is influenced only by solutes that cannot cross the membrane, as only these exert an osmotic pressure. Solutes able to freely cross the membrane do not affect tonicity because they will always be in equal concentrations on both sides of the membrane. There are two things to always remember about osmoses and tonicity: Tonicity is always in comparison to a cell. The cell has a specific amount of sugar and salt

Remember the three key terms: A Hypertonic solution has more solute (so LESS water) than the cell. A cell placed in this solution will give up water (osmosis) and shrink. A Hypotonic solution has less solute (so MORE water) than the cell. A cell placed in this solution will take up water (osmosis) and expand. An Isotonic solution has just the right amount of solute for the cell. A cell placed in this solution will stay the same. An example of the effects of each of these osmotic environments on a typical plant cell is shown in Figure 1. Osmosis has different effects on different species ]In animal cells, a hypertonic environment forces water to leave the cell so that the shape of the cell becomes distorted and wrinkled, a state known as crenation. In plant cells, the effect is more dramatic. The flexible cell membrane pulls away from the rigid cell wall, but remains joined to the cell wall at points called plasmodesmata. The cell takes on the appearance of a pincushion, and the plasmodesmata almost cease to function because they become constricted a condition known as plasmolysis. In plant cells the terms isotonic, hypotonic and hypertonic cannot strictly be used accurately because the pressure exerted by the cell wall significantly affects the osmotic equilibrium point. Figure 1 The effect on plant cells under different osmotic environments.

Some organisms have evolved intricate methods of circumventing hypertonicity. For example, saltwater is hypertonic to the fish that live in it. They need a large surface area in their gills in contact with seawater for gas exchange, thus they lose water osmotically to the sea from gill cells. They respond to the loss by drinking large amounts of saltwater, and actively excreting the excess salt. This process is called osmoregulation. In a hypotonic environment, animal cells will swell until they burst, a process known as cytolysis. Fresh water fish urinate constantly to prevent cytolysis. Plant cells tend to resist bursting, due to the reinforcement of their cell wall, which provides effective osmolarity or osmolality. In some cases of suspensions intended for intramuscular injection, a slightly hypotonic solution is preferred in order to increase the dissolution and absorption of the drug by absorbing water from the surrounding tissues. OBJECTIVES for week one: During this lab, you should be able to: 1. Determine the effect of molecular mass on the diffusion rate of particles through a media. 2. Measure the osmotic pressure in cells of a potato using a gradient of solutions. Solution preparations: You will be provided with a 0.2 M stock solution of sodium chloride (NaCl) and firstly you will learn how to calculate dilutions for varying molar solutions Calculating and making 10 ml of varying molar solutions from 0.2 M NaCl: First, calculate amount of stock solution (0.2M NaCl needed) to reach desired dilution Molar Solution needed in dilution X 10 ml = ml of 0.2 M NaCl 0.2 M e.g. to dilute a 0.2M NaCl (stock solution) to a 0.15 M NaCl (desired dilution) (0.15M X 10 ml)/0.2m = 7.5 ml of 0.2M NaCl Second, calculate the amount of dh 2 0 is needed to bring it up to 10 ml

Put these amounts in table below and calculate amounts of stock solution and dh20 needed to dilute to 0.1M and 0.05M solutions. 0.2 M NaCl dh 2 0 dh 2 0 0 ml 10 ml 0.2 M 10 ml 0 ml 0.15 M 7.5 ml 2.5 ml 0.10 M 0.05 M 0.025 M e.g. for a 0.15 Molar of NaCl in 10 ml, we need 7.5 ml of 0.2M NaCl and 2.5 ml of dh 2 0 Make above solutions and put into test tubes a. Using a cork borer cut cylinders from a single potato (the cuts are made parallel). b. A razor blade is used to cut the ends of the potato cylinders square (all cylinders are equal in length). A length of about 30 mm gives good data. c: All cylinders of potato must be equal in length, width, and appearance. d. Measure and record the length and weight of each potato cylinder. All measurements must be similar. e. Place a potato cylinder into a test tubes. f. Each of the test tubes is labeled and filled about 2/3 full with a different one of the salt solutions. g. Weigh the potato cylinders after 10 mins and every 10 mins up to about 1 ½ hours. Then remove the potato cylinders from the test tubes. dh20 0.2M 0.15M 0.10M 0.05M 0.025M 1 2 3 4 5 6 Average Plot the average values in Excel. Plot change in cell size over time

Things to define: Diffusion Osmosis Solute Solvent solution hypertonic Solution Week two: What else would govern osmosis movement in an environment? Is it just salt concentration:? Does sugar content play a part? Remember the plant cell would be full of sugar due to the process of photosynthesis. What about temperature? Design next week s experiment to govern these parameters. Hand in a plan for your group experiment at the end of today s lab. What other parameters will you be investigating, and how. Do you want to use a different plant material and why Week three: As a lab group: Mini PowerPoint presentation on osmosis in plant cells. Have a print out of your presentation and this lab brief to hand in then.