ASEPTIC TECHNIQUES TO BE OBSERVED IN THE LABORATORY 1.

Wear a protective gown made of material easily cleaned and sterilized if possible and avoid wearing this outside to prevent possible spread of contaminants to the outside. 2. Disinfect you working area before and after use. 3. Disinfect your hands before each and after each laboratory manipulations. 4. Avoid putting anything in your mouth during laboratory exercises. 5. Always flamed-sterilized forceps, rods, loops and needles before laying them aside. 6. Avoid any kind of contaminated materials from spilling and contacting surfaces, hands from spilling and contacting surfaces, hands or clothing. Notify the laboratory instructor immediately if accidents happen even a minor one. 7. Keep personal items in place designated and away from working area. 8. Arrange culture and infectious materials in a secure place of the table. Do not allow unused equipment to accumulate in your working area. 9. Dispose infectious materials/cultures and contaminated materials carefully as prescribed by the instructor. Note location of special containers for disinfectants used regularly. 10. Keep glasswares and equipment clean and in their proper place. Be as clean and as orderly as possible at all times. LABORATORY PROCEDURES 1. Keep laboratory manual on hand. Read the procedure thoroughly before you start with the exercise. Always think and plan ahead. 2. Keep only equipment/materials in use on the table. Be careful in handling them. They are expensive. 3. Perform the exercise. Pay attention to the preliminary briefing of your instructor. Check and ask your instructor for clarification. Take note of your results and records all measurements and observations. 4. Label your culture and study specimens as indicated by your instructor. Include the following data: Name or initials Name of organisms Culture media used Date of culture

5. Use references. Check related materials in textbooks and outside references. Make conclusion about the data you have gathered. How does it relate to the works done in the field? Have other problems been raised by the data your exercise generated? 6. Dispose of contaminated and infectious materials. Locate proper jars and pans for discards. Heat them to boiling before discarding. 7. Replace equipment, glassware and materials where you find them. 8. Turn off the water, light and gas outlet when not in use. MATERIALS AND SUPPLIES NEEDED Each student is required to bring the following: Laboratory Gown Face masks Hand towel Disposable gloves Data notebook Gatorade bottles Scissors Glass marking pens/pencils Millimeter rule Gum labels Detergent Cotton/gauze Aluminum foil polypropylene plastics ethyl alcohol tissues matches millimeter ruler Matches

LABORATORY EXERCISE NO. 1 MICROSCOPY INTRODUCTION The microscope is one of the indispensable tools of biologists in observing and probing the structural basis of life. Microscopy is the techniques used designed to help you become familiar with and proficient in the use of microscope. This consists of a system of lenses and appropriate mechanical fixtures for focusing and observing live or stained specimens. The objective lenses are close to the object and produce magnified image of it. The ocular lenses are near the eye and magnify the image. Magnification is the enlargement of the image and is the end result of the combined effects of the objective and ocular lens system. The objective lens provides an enlarge image of the object from 4 to 100x and the ocular lens magnify the image n more than 10 to 15 times. The total magnification of the lens system is the product of the objectives magnification and the oculars magnification. The resolution of a bright field microscope is defined as the ability of lens system to produce an image that allows the viewer to distinguish between two structures near each other in a specimen. The resolving power of the microscope is determined by the wavelength of light used to illuminate the object, index of refraction between the specimen and objective lens and half the angle of the cone of light entering the lens. The testing, calibration and critical use of a microscope demands a precise alignment of all optical components For microscopic observations to have meaning, one must have a standard means of measurement and a way to determine the size of the specimen under investigation. The metric system has been adopted by the scientific community in order to establish a uniform standard of measurements and is now used by most scientists for all quantitative determinations (Appendix A, Table 1) OBJECTIVES 1) To explain how various types of microscopes work and their importance in the field of microbiology. 2) To let the students understand the principles involved in order that the instrument maybe employed to greater advantage. 3) To impress to the students the importance of proper care and maintenance of such precision instrument.

METHODOLOGY Parts of the Microscope Place the microscope in proper position. Locate all parts and learn the functions of each.

Fiigure 1. The compound microscope A. Manipulation of Microscope 1) Specimens to be examined under the microscope a. Alga (Spirulina sp) b. Fungus (Saccharomyces cereviseae) c. Protozoa (Epistylis) d. Bacteria (Staphylococcus aureus) 2) Focus the specimen with the 4x or 10x objectives. Adjust the eyepieces of the microscope to your own personal measurements. Look through the eyepiece and adjust the distance between the eyepieces until one circle of light appears. 3) Close the iris diaphragm so only a minimum of light enters the objective lens.

4) Lower the condenser until a distinct circle of light is visible. Open the iris diaphragm until the light just fills the field. 5) When an image has been brought into focus with low power and have completed your observations, swing the high dry objective into position and focus. The specimen will remain almost in focus and only slight adjustment is needed. You may need more light for better resolution. 6) Move the high dry out of position and place a drop of immersion oil on the area of the slide you are observing. Carefully click the oil immersion lens into position. Focus with the fine adjustment. When observations are completed swing back to low power objective and clean the objective with lens paper. Remove the slide. Repeat the procedure with other specimens. B. Calibration of the Microscope Microscope objects can be measured by means of ocular micrometer. Both must be calibrated first with stage micrometer. 1) Remove the eyepiece from the drawtube and replace it with the micrometer eyepiece. 2) Place the micrometer stage in the stage and focus in its scale. Arrange the stage micrometer so that one line in it coincides with the line in the ocular. 3) Count the number of divisions in the ocular micrometer coinciding with line in the stage scale. 4) Count the number of divisions in the ocular micrometer subtended by the number of divisions in the stage micrometer. It is important that the line coincides properly. 5) Use the following formula to determine the value of one division in the ocular micrometer.
stage micrometer division value of one stage subtended by ocular micrometer x micrometer divisions (m)

F=
ocular micrometer divisions subtended by stage micrometer

6) Measurement of the specimen 7) Measure the specimen by counting the number of divisions it will cover in the ocular micrometer. Compute the size of the specimen using the calibration factor.
8) Care of the microscope. Clean the microscope after using. Be sure to remove the oil

from the oil immersion objective. Use lens paper only on optical glass parts (objective).

RESULTS AND DISCUSSION Guide Questions for Discussion 1) How can each objective be identified if identification marks are removed? 2) As you go from the low power to the high power what happens to the: a) Diameter of the field of vision b) Amount of light reaching your eye c) Working distance between lens and slide 3) Explain the use of scanning, low power, high dry and oil immersion objectives. What characteristic of the microscope makes it possible to switch from one objective to another and still be in focus? 4) What is the numerical aperture of a lens? What are its functions? 5) Define resolving power of a microscope. How can you use this to better advantage? 6) Why oil often put between stained specimens and the objective lens? 7) Of what use is a dark-field microscope? Why are the field dark and the object light? 8) Of what use is the phase-contrast microscope? Explain why small objects are dark compared to bright field. 9) Of what use is the fluorescence microscope? What kind of light is used to illuminate the specimen? Explain why the field is dark and the object colored? 10) Computation of Drawing Magnification a) Draw your specimen in a 10 x 10 cm square. Using the actual size of your specimen compute for your drawing magnification by dividing the size of your drawing by the actual size of your specimen REFERENCES:

LABORATORY EXERCISE 1

MICROSCOPY

Name: Date Performed Rating:

RESULTS 1. Complete the following table. OBJECTIVE NUMBER OF DIVISIONS OCULAR STAGE CALIBRATION FACTOR (CF) STAGE OCULAR

2. Determination of the Diameter and Area of the Field of Vision DIAMETER (mm) RADIUS mm m MEAN AREA mm2 m2

OCULAR

OBJECTIVES

Why should the ocular micrometer be calibrated for each object? Can a calibrated ocular micrometer measure the diameter of a field? Why or why not? 3. Determination of the Width and length of the specimen DIAMETER OF THE FIELD (LPO) mm m ESTIMATE WIDTH OF SPECIMEN mm m

4. Magnification Draw the representative specimen from each slide and show how they appeared at each magnification. Note the differences in size of the algae, bacteria, fungi and protozoa at each magnification.