Laboratory 3 Organic Molecules

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1 Laboratory 3 Organic Molecules MATERIALS Distilled water, vegetable oil, and solutions of glucose, starch, and gelatin Dairy products (half and half, heavy cream and whole milk) Non-dairy soy and almond milk The biuret reagent, and NaOH IKI (iodine potassium iodide or Lugol s iodine solution) Benedict s reagent Sudan IV/glycerol solution 70% ethanol White ceramic spot plates, china markers (grease pencils), toothpicks, and eyedroppers Pipettes, test tubes, test tube racks, and test tube holders Thin tissue sections cut from bean, potato, and almond plants Tweezers, microscope slides, cover slips, and a No. 2 pencil 100 C water bath, 4 C ice bath, and vortex mixer LEARNING OUTCOMES Upon completion of the exercises in this laboratory, you should be able to: 1. Use the appropriate biochemical tests to determine the presence of three types of organic molecules 2. Distinguish the positive from negative outcomes for each biochemical test 3. Establish a hypothesis 4. Collect and interpret results 5. Identify the specific type of milk being tested based upon the organic molecules it contains Living organisms are composed of four large groups of organic molecules: carbohydrates, proteins, lipids, and nucleic acids. Each has a specific biologic role, and very often a specific distribution within a living organism. A knowledge of an organic molecule s chemical properties, functions, and interactions are fundamental to understanding cellular processes. Therefore, the detection of organic molecules in laboratory tests is a necessary part of the study of organisms. Over the past centuries, specific biochemical tests have been developed to detect organic molecules, some of which will be used in this and future laboratory exercises. The identification of organic molecules is also useful in the analyses of the composition of foods derived from both plants and animals. The organic molecules found in foods vary depending on their source and post-harvest processing. Many food products are modified from their native states to satisfy the needs of consumers. For example, lactose intolerant individuals cannot process lactose (a disaccharide of glucose and galactose) leading to problems in their digestive tracts. Manufacturers of dairy products market lactose free milk to eliminate these problems. Manufacturers also manipulate the amount of lipids in milk to range from fat free (0% lipid) to whole (~3.2% lipid). Confusingly, several plant-based (non-dairy) milks are also available to consumers including almond and soy milk. We can compare the organic molecules of dairy vs. non-dairy milks. In this laboratory, several milks and other solutions will be tested to identity their constituent organic molecules. 1 B IO 150 Laboratory 3

2 Appropriate laboratory techniques and procedures must be followed for accurate results. Scientific procedures, similar to cooking recipes, require care and precision for a successful outcome. In addition, laboratory tests must include both positive and negative controls to establish their validity. To identify organic molecules, a positive control illustrates a specific (positive) result with a known molecule. A negative control will lack any molecules that will generate this positive result. In our experiments, a negative control often substitutes water for other molecules. A positive reaction will involve a visible change in the color of a solution inferring that a particular organic molecule is present within it. The controls thus establish reference points for all the reactions performed on solutions with unknown compositions. Separate tests will be performed to detect the presence of proteins, carbohydrates, or lipids. Questions 1. Does milk processing influence its constituent organic molecules? 2. Do non-dairy and dairy milk contain the same organic molecules? 3. Can specific tests performed in this laboratory distinguish between dairy products? The samples to be analyzed include whole milk, heavy cream, half and half, almond milk, and soy milk. Based upon previous knowledge, establish a hypothesis for each question above and provide a rationale for it: Hypotheses Rationales B IO 150 Laboratory 3

3 Note that each specific test will require a positive and negative control. Water and separate solutions containing glucose (a simple sugar or monosaccharide), starch (a polymer sugar or polysaccharide), gelatin (a mixture of proteins, mainly collagen) and vegetable oil (lipids) will be provided. Exercise 3.1 Detection of Lipids (Sudan IV Test) Lipids (fats and oils) are the most prevalent component of most organisms. Lipid molecules, due to their non-polar bonds, are hydrophobic (lipophilic) and as such do not readily mix with water. They are soluble in various organic solvents including ethanol, hexanes, and ether. Phospholipids, followed by cholesterol (also a lipid) are the major components of cell membranes. Cholesterol tends to stiffen most cellular membranes. Cholesterol is also the parent component for the production of steroids (i.e.; testosterone, estrogen, cortisol). The major fats of both animals and plants, in structures known as triglycerides, are used to store energy. Curiously, hydrophobic lipids are commonly found within watery cells or the watery fluid that surrounds cells. One would expect the lipids to be separated from the watery environments due to their hydrophobicity. Using internet resources, try to use relevant information to establish a hypothesis about how lipids are maintained within these hydrophilic environments. Hypothesis Most biochemical tests to detect lipids rely upon lipophilic (lipid soluble) reagents. Sudan IV is a lipophilic substance that when mixed with lipids stains them red. 3 B IO 150 Laboratory 3

4 Procedure 3.1 Detecting Lipids with Sudan IV 1. Obtain an appropriate number of test tubes and place them in a rack on your laboratory bench. Label the tubes with a china marker (grease pencil). 2. Pipette 1 ml of distilled water into one test tube, and the same amount of each solution listed in Table 3.1 to a separate, appropriately labeled test tube. Use a separate pipette for each solution. Distilled water can also be obtained directly from its container. 3. Add 10 drops of the Sudan IV/glycerol solution to each test tube and gently mix the contents with a vortex mixer for about 5 seconds. 4. Allow the tubes to remain within an undisturbed rack for 5 minutes. It might be necessary to place the tubes in an ice bucket for better results. 5. The appearance of a red layer within the solution infers the presence of lipids. Use the negative control for comparison and record the visual results in Table 3.1. Note any difference in the intensity of the red color. Observe the results again after the incubation of the tubes on ice. 6. Discard the contents of the test tubes in a sink, wash them thoroughly with soap and tap water, rinse them extensively with tap water, and place them inverted in a test tube rack to dry upon your laboratory bench. Table 3.1 Detection of Lipids (Sudan IV Test) Results Tube # Solution Final Color 1 Water 2 Glucose 3 Starch 4 Gelatin 5 Vegetable oil 6 Milk A 7 Milk B 8 Milk C 9 Milk D 10 Milk E Presence (+) or Absence ( ) of Lipids 4 B IO 150 Laboratory 3

5 Exercise 3.2 Detection of Proteins Proteins are polymers of specific arrangements of 20 amino acids linked together by peptide bonds. An enormous number of proteins can be synthesized through different combinations and numbers of amino acids. This diversity leads to numerous cellular functions for proteins including structural (i.e.; within the cytoskeleton and extracellular matrix) and functional (i.e.; enzymatic, hormonal, secretory) roles. Peptide bonds are a unique chemical feature within proteins that separate them from other organic molecules. They are formed by a dehydration synthesis (polymerization reaction) that generates a covalent bond between two amino acids. The peptide bond is specifically between the carbonyl (C=O) group on one amino acid and the amine group (N-H) of another (marked with a * in Figure 3.1). * Figure 3.1 Peptide Bond Formation A specific test to detect proteins is known as the biuret reaction in which a blue solution containing copper sulfate (CuSO 4 ) changes to a violet color in the presence of two or more peptide bonds. A simplification of the reaction is illustrated in Figure 3.2. Figure 3.2 The Biuret Reaction The solutions listed in Table 3.2 will be tested for the presence of proteins utilizing the biuret reaction. 5 B IO 150 Laboratory 3

6 Procedure 3.2 Detecting Proteins (Biuret Reaction) 1. Obtain a white ceramic spot plate, the biuret reagent, eyedroppers, and the solutions listed in Table Number the wells of the spot plate with a china marker (grease pencil). 3. With the supplied eyedroppers, add 5 drops of distilled water in one well, and 5 drops of each organic solution listed in Table 3.2 to separate appropriately labeled wells. Use a separate eyedropper for each solution. Drops of distilled water can also be obtained directly from its container. 4. Add 3 drops of the biuret reagent into each well of the spot plate and mix the contents with a toothpick. Use a separate toothpick for each individual well. 5. After mixing, the appearance of violet color in a well indicates the presence of protein. Use the negative control for comparison and record the visual results in Table Discard the contents of all wells of the spot plate in a sink, rinse the plate with tap water, and dry it with a paper towel. Use the cleaned plate in the next exercise. Table 3.2 Biuret Reaction Results Review Well # Solution Final Color 1 Water 2 Glucose 3 Starch 4 Gelatin 5 Vegetable oil 6 Milk A 7 Milk B 8 Milk C 9 Milk D 10 Milk E Presence (+) or Absence (-) of Protein What were your negative and positive controls and what were their functions in the experiment? The biuret test is specific for proteins because: 6 B IO 150 Laboratory 3

7 Exercise 3.3 Detection of Starch (IKI Test) Starch represents one of several polysaccharides composed of a single type of monosaccharide (simple sugar) known as glucose. Glucose monomers (single molecules) are the main source of energy for most cells. Cells store excess glucose by linking it together via glycosidic bonds (a type of covalent bond) forming polymers (chains of linked monomers) known as plant starch or animal glycogen. Saccharides and polymers of saccharides are collectively known as carbohydrates. Structurally, the starch molecule is a coiled and spring-like polymer of glucose. To detect starch in a substance one can add iodine (IKI or Lugol s iodine solution) to it. Iodine molecules can slide into and accumulate within coils of starch. Solutions of free iodine are dark amber (yellowbrown) in color. When iodine is concentrated within coils, a blue-black color develops, inferring the presence of starch (see Figure 3.3). Figure 3.3 Iodine (purple spheres) Accumulating in Starch (connected white hexagons) Procedure 3.3 Detecting Starch (IKI Test) 1. Use the cleaned white spot plate from the previous exercise. Determine how many wells will be needed and label them with a china marker (grease pencil) appropriately. 2. With the supplied eyedroppers, add 5 drops of water in one well, and 5 drops of each solution listed in Table 3.3 to separate appropriately labeled wells. Use a separate eyedropper for each solution. Drops of distilled water can also be obtained directly from its container. 3. Add 1 drop of the IKI solution into each of the wells of the spot plate and mix the contents with a toothpick. Use a separate toothpick for each solution. 4. The appearance of a blue-black color indicates the presence of starch. Use the negative control for comparison and record the visual results in Table Discard the contents of the spot plate in a sink, rinse it with tap water, and dry it with a paper towel. 7 B IO 150 Laboratory 3

8 Table 3.3 IKI Test Results Well # Solution Final Color 1 Water 2 Glucose 3 Starch 4 Gelatin 5 Vegetable oil 6 Milk A 7 Milk B 8 Milk C 9 Milk D 10 Milk E Presence (+) or Absence ( ) of Starch Review Starch is a polysaccharide carbohydrate. Will IKI react with all carbohydrates? Explain. Which numbered well can be used to explain the answer to the previous question? Why? 8 B IO 150 Laboratory 3

9 Exercise 3.4 Detection of Reducing Carbohydrates (Benedict s Test) The building blocks of di- and polysaccharides are the so-called simple sugar monosaccharides (i.e.; glucose, fructose, and galactose). In the body, dietary monosaccharides are absorbed without modification and are later converted to glucose within the liver. In addition, dietary carbohydrates include di- and polysaccharides that are enzymatically digested to monosaccharides before cellular absorption. The common disaccharides include maltose (glucose glucose), sucrose (glucose fructose) and lactose (glucose galactose). Monosaccharides and some disaccharides (known as reducing sugars) can be detected by a test utilizing another copper-based solution known as Benedict s reagent. * This method relies upon the ability of reactive (reducing) mono- and disaccharides to donate electrons to Cu ++ ions of Benedict s reagent. In solution, when Cu ++ gains a negative electron it becomes (reduces to) Cu + and a color change from blue to brick-red is observed. Specifically, the color of a positive test can range from green (low sugar concentration), to orange-brown (moderate sugar concentration), and to brick red (high sugar concentration). A simplified version of the reaction is illustrated in Figure 3.4. reducing sugar Benedict s reagent (blue) oxidized sugar reduced Benedict s reagent (red) Figure 3.4 Reduction of Benedict s Reagent by a Sugar Molecule Procedure 3.4 Detecting Reducing Sugars (Benedict s Test) 1. Obtain an appropriate number of test tubes and place them in a rack on your laboratory bench. Label the tubes with a china marker (grease pencil). 2. Add 1 ml (or 20 drops with an eye dropper) of water into one test tube, and the same amount of each solution listed in Table 3.4 to separate and appropriately labeled test tubes. Use a separate eyedropper for each solution. Drops of distilled water can also be obtained directly from its container. 3. Add 1 ml of the Benedict s reagent to each test tube and gently mix the contents with a vortex mixer for about 5 seconds. 4. Place all the test tubes within a 100 C water bath for 5 minutes. 5. Carefully remove the hot tubes individually from the water bath using a test tube holder, place them in a test tube rack, and bring them back to your laboratory bench. * Benedict, S.R. (1909). A reagent for the detection of reducing sugars. Journal of Biological Chemistry 5: BIO 150 Laboratory 3

10 6. The appearance of a green, orange, or brick-red solution infers the presence of reactive (reducing) mono- or disaccharides. Use the negative control for comparison and record the visual results in Table 3.4. Note that each specific color corresponds to an overall concentration of reducing mono- and disaccharides within each solution. 7. Discard the contents of the test tubes in a sink, wash them thoroughly with soap and tap water, rinse them extensively with tap water, and place them inverted in a test tube rack to dry upon your laboratory bench. Table 3.4 Detection of Reducing Sugars (Benedict s Test) Results Tube # Solution Final Color 1 Water 2 Glucose 3 Starch 4 Gelatin 5 Vegetable oil 6 Milk A 7 Milk B 8 Milk C 9 Milk D 10 Milk E Presence (+) or Absence (-) of Reducing Sugar Review The Benedict s test detects glucose, the building block of starch, yet it does not detect starch. Explain. Starch is consumed while eating french fries. What process can generate glucose molecules from this starch? Which types of molecules carry out that process? What human disease could be monitored by Benedict s test? What might be the easiest way to do this? 10 B IO 150 Laboratory 3

11 Summary of Organic Molecules Detected Within Milks Based upon the tests performed, and the data recorded in Tables , determine the content of the milks listed in Table 3.5. Try to identify the type of milk (i.e.; whole milk, heavy cream, half and half, almond, or soy) of each based upon the organic molecules found within them. Table 3.5 Organic Molecules Detected within Milks Results Milk Milk A Milk B Milk C Milk D Milk E Biuret Reaction (+/ ) IKI Test (+/ ) Benedict s Test (+/ ) Sudan IV Test (+/-) Organic Molecules Detected Sample Identity Address the validity of each of the three hypotheses you proposed at the beginning of this laboratory and explain your conclusions Which of the milks tested will probably provide the most diverse nutrition? Individuals performing physically demanding activities requires significant amounts of proteins and carbohydrates. If only vegetables are available, what will a menu for these individuals need to be supplemented with? 11 B IO 150 Laboratory 3

12 Exercise 3.5 The Detection of Organic Molecules Within Tissues Organic molecules can be detected within specific areas of cells, or within specific tissues, using the reagents of the previous exercises. Color changes (staining) can be microscopically (histologically) observed within cells or tissues inferring the presence and location of specific organic molecules. In a prior laboratory, a prepared permanent microscopic sample containing a subspecies of Paramecium were observed. In addition to permanent slides, microscopic slides can be prepared from fresh living tissues (known as wet mounts). Wet mounts are usually intended for immediate observation and cannot be preserved for longer periods of time. The preparation of a wet mount is relatively simple. A thin tissue section is placed upon a microscope slide, and a drop of water, or staining reagent, is added over the specimen. A small coverslip is then slowly lowered from a 45 o angle over the sample (see Figure 3.5). Excess water and/or staining reagents that leaks outside of the edges of the coverslip can be gently wicked away with the edge of a paper towel. Figure 3.5 Preparation of a Wet Mount Slide 12 B IO 150 Laboratory 3

13 Preparation and Staining of Living Plant Tissues Wet-mounts will be prepared from potato (Solanum tuberosum), white beans (Phaseolus vulgaris), and almond (Prunus dulcis) tissues. Each will be stained separately with an IKI solution, the Biuret reagent, and Sudan IV. After the staining procedures, coverslips are discarded as glass trash, but slides can be rinsed free of tissues with tap water and reused. Procedure 3.5 IKI Staining 1. Obtain 3 clean microscope slides and label them within their frosted areas with a pencil. 2. Thin sections of each sample will be cut from each plant (your instructor will describe the procedure and provide the sections). Add 1 drop of distilled water to each section laid upon the center of a slide. Slowly lower a coverslip from a 45 o angle over the section to complete the wet mount. Remove any excess fluid with a paper towel before placing the slide on the microscope stage. 3. Observe the wet mount under the microscope with low (40X) and then high (400X) magnification. Sketch each tissue in Figure Carefully add 1 drop of IKI to one edge of the coverslip. It should mix with the water under the coverslip, but the stain can also be drawn under by briefly applying a paper towel to the opposing edge of the coverslip. Observe this wet mount under the microscope as in the previous step. Draw your observations in Figure 3.7. Procedure 3.6 Biuret Staining 1. You will be provided with thin sections from potato, bean, and almond tissues. 2. Transfer the sections with a tweezers into separate wells of a white spot plate and then add 2 drops of NaOH to each and incubate for 5 minutes. 3. Add 1 drop of CuSO4 to each well and gently agitate the plate with a circular motion on the bench. 4. Transfer the sections onto slides with a tweezers and then generate wet mounts for observation under the microscope. Draw your observations in Figure B IO 150 Laboratory 3

14 Procedure 3.7 Sudan IV Staining 1. You will be provided with thin sections from potato, bean, and almond tissues. 2. Transfer the sections with a tweezers into separate wells of a white spot plate and cover each with 3 drops of the Sudan IV/glycerol solution. Allow the sections to stain for about 5 minutes. 3. Transfer the sections independently to other wells within the spot plate with tweezers and then cover with 10 drops of 70% ethanol. Gently agitate the plate for about 30 seconds. This step washes away excessive Sudan IV. 4. Transfer the sections independently to a third set of wells of the spot plate with a tweezers and then cover with 10 drops of distilled water as a final rinse. 5. Transfer the sections onto slides with a tweezers and then generate wet mounts for observation under the microscope. Draw your observations in Figure 3.9. Potato Bean Almond Figure 3.6 Unstained Tissue Sections at 400X Figure 3.7 IKI Stained Tissue Sections at 400X 14 B IO 150 Laboratory 3

15 Potato Bean Almond Figure 3.8 Biuret Stained Tissue Sections at 400X Review Figure 3.9 Sudan IV Stained Tissue Sections at 400X Which of the tissues stained positively for starch? For proteins? For lipids? Can you localize any of the organic molecules to specific organelles within the cells you observed? If so, what organelles stained positively for starch, proteins, or lipids? 15 B IO 150 Laboratory 3

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