Preparation of a Bacterial Smear and the Simple Stain Technique

Preparation of a Bacterial Smear and the Simple Stain Technique

© Jones & Bartlett Learning, LLC © Jones & Bartlett Learning, LLC NOT FOR SALE OR DISTRIBUTION NOT FOR SALE OR DISTRIBUTION Preparation © Jones & Bartlett Learning, LLC © Jones & Bartlett Learning, LLC NOT FOR SALEof OR a DISTRIBUTION Bacterial NOT FOR SALE OR DISTRIBUTION Smear and the © Jones & Bartlett Learning,Simple LLC Stain© Jones & Bartlett Learning, LLC NOT FOR SALE OR DISTRIBUTIONTechnique NOT FOR SALE OR DISTRIBUTION © Jones & Bartlett Learning, LLC © Jones & Bartlett Learning, LLC NOT FOR SALE OR DISTRIBUTION NOT FOR SALE OR DISTRIBUTION ost bacteria have no color, so they generate little contrast in the microscope field. Therefore, to see bacteria with the micro- M scope, it is necessary to apply color by using a staining reagent. Once ©stained, Jones the & Bartlett bacteria Learning, may be observed LLC and studied with© Jones & Bartlett Learning, LLC respect to theirNOT shape, FOR size, SALE and arrangement. OR DISTRIBUTION NOT FOR SALE OR DISTRIBUTION The preparation of a stained bacterial smear involves several steps. First, bacteria are placed on a glass slide and “fixed” with heat, partly to ensure that they remain attached to the glass. Then, for simple staining, a basic© Jones stain & is Bartlett applied. Learning,Such a stain LLC carries a positive electrical© Jones charge. & TheBartlett Learning, LLC negativelyNOT FOR chargedSALE OR surface DISTRIBUTION and cytoplasm of bacteria attractsNOT FOR the stain,SALE OR DISTRIBUTION and staining takes place. In this exercise, we shall explore the proper meth- ods for simple staining. The technique is called the simple stain technique because only a single stain is used. Other staining techniques are explained in Exercises 5, 6, and 7. © Jones & Bartlett Learning, LLC © Jones & Bartlett Learning, LLC NOT FOR SALEThis OR DISTRIBUTIONexercise also will demonstrate theNOT important FOR SALE techniques OR DISTRIBUTION for handling bacterial cultures. Each is a “pure culture;” it contains only one species of bacterium. The bacteria have been cultivated in a liquid growth medium such as nutrient broth or on a solid growth medium such as nutri- ent agar. Your instructor will specify the medium used. © Jones & Bartlett Learning, LLC © Jones & Bartlett Learning, LLC NOT FOR SALE OR DISTRIBUTION NOT FOR SALE OR DISTRIBUTION A. Preparation of a Bacterial Smear © Jones & Bartlett Learning, LLC © Jones & Bartlett Learning, LLC NOT FOR SALE OR DISTRIBUTION NOT FOR SALE OR DISTRIBUTION A bacterial smear is a thin layer of bacteria placed on a slide for staining. PURPOSE: to prepare a bac- Preparing the smear requires attention to a number of details that help terial sample for staining. prevent contamination of the culture and ensure safety to the preparer. Each step in this procedure has an important reason, and each should be fol- © Jones & Bartlett Learning, LLC © Jones & Bartlett Learning, LLC lowed carefully as a prerequisite to successful work. NOT FOR SALE OR DISTRIBUTION NOT FOR SALE OR DISTRIBUTION © Jones & Bartlett Learning, LLC. NOT FOR SALE OR DISTRIBUTION.5054 © Jones & Bartlett Learning, LLC © Jones & Bartlett Learning, LLC NOT FOR SALE OR DISTRIBUTIONS pecial Materials NOT FOR SALE OR DISTRIBUTION • Pure cultures of selected bacterial species © JonesP &rocedure Bartlett Learning, LLC © Jones & Bartlett Learning, LLC NOT FOR1. BeginSALE this OR exercise DISTRIBUTION by disinfecting the laboratory deskNOT with FORthe available SALE dis- OR DISTRIBUTION infectant as directed by the instructor. Then place a clean sheet of paper tow- eling or other absorbent material over the area to be used. Should a spill occur, the paper will absorb the liquid and can be disposed of as directed by the instructor. © Jones & Bartlett Learning, LLC © Jones & Bartlett Learning, LLC NOT FOR SALE OR DISTRIBUTION2. Wash a glass slide with soap, rinse itNOT well, FORand dry SALE it thoroughly, OR DISTRIBUTION preferably with a lint-free cloth. With a wax marking pencil or felt marker, mark off areas of the slide where smears will be placed. One area should be reserved for a slide label. Some laboratory workers prefer to use the underside of © Jones & Bartlett Learning, LLC the slide for marking© Jonesto prevent & waxBartlett from Learning,mixing with LLCthe smear. Others use the top because the wax barrier holds the dye in that area and prevents NOT FOR SALE OR DISTRIBUTION NOT FOR SALE OR DISTRIBUTION spreading. 3. Obtain cultures of the bacteria, and place the tubes in a suitable rack on the bench. Sterilize your inoculating loop. If agar slant cultures are used, © Jones &place Bartlett a loopful Learning, of water intoLLC one area of the slide. If broth© Jones cultures & Bartlett are used, Learning, LLC no additional liquid is necessary. Light the Bunsen burner. The smear is NOT FOR SALE OR DISTRIBUTION NOT FOR SALE OR DISTRIBUTION now ready to be prepared. Review the transfer procedure outlined in Exercise 1. When lighting the Bunsen 4. Referring to Figure 1A, firmly hold the loop as you would hold a pencil, and burner for use in the lab place it nearly vertically into the blue tip portion of a Bunsen burner flame for be sure© to Jonesface it away & Bartlett Learning, LLC © Jones & Bartlett Learning, LLC a few seconds or until it glows red hot. Allow the loop to cool several seconds. from you.NOT FOR SALE OR DISTRIBUTION NOT FOR SALE OR DISTRIBUTION 5. Take the bacterial culture in the opposite hand, remove the cap as shown in Figure 1B. Place the tip of the tube in the flame for a few seconds (Figure 1C). ! This will burn off any dust or lint and kill any airborne organisms that might happen to fall into the tube. © Jones & Bartlett Learning, LLC © Jones & Bartlett Learning, LLC NOT FOR SALE OR DISTRIBUTION6. Insert the loop into NOTthe tube, FOR and SALE touch itOR very DISTRIBUTION gently to the main portion of the slant (Figure 1D). Be careful not to dig into the medium or scrape it. Quick Procedure If a broth medium is used, dip the loop carefully into the liquid. Remove the Smear loop, reflame the tip of the tube briefly (Figure 1E), then replace the cap Preparation (Figure 1F), and return the culture to the rack on the desk. © Jones & Bartlett Learning, LLC © Jones & Bartlett Learning, LLC 1. Label a clean micro- 7. Mix the loopful of bacteria with the loopful of water on the slide (Figure 1G), scope slide. NOT FOR SALE OR DISTRIBUTION NOT FOR SALE OR DISTRIBUTION and swirl the liquid out to the area of a dime. For broth cultures, simply 2. Sterilize the inoculating swirl the loopful of bacteria on the marked slide area. Complete the proce- loop. dure by reflaming the loop (Figure 1H). You now have a bacterial smear. 3. Remove a bacterial or broth© Jones sample. & Bartlett Learning,8. Prepare LLC other smears in the remaining© Jones spaces & withBartlett different Learning, bacteria LLC as NOT FOR SALE OR DISTRIBUTIONdirected by the instructor. It is importantNOT thatFOR you SALE become OR comfortable DISTRIBUTION with 4. Smear on slide area. the methods for handling cultures and preparing smears since they are 5. Air dry. essential elements of laboratory microbiology. Your instructor may recom- 6. Heat fix. mend other sources to be examined, as specified in the next part of this exercise, Part B, step 6. All smears on one slide should be prepared before pro- © Jones & Bartlett Learning, LLC © Jones & Bartlett Learning, LLC ceeding with the next step. NOT FOR SALE OR DISTRIBUTION NOT FOR SALE OR DISTRIBUTION © Jones & Bartlett Learning, LLC. NOT FOR SALE OR DISTRIBUTION.5054 © Jones & Bartlett Learning, LLC © Jones & Bartlett Learning, LLC NOT FOR SALE OR DISTRIBUTION NOT FOR SALE OR DISTRIBUTION © Jones & Bartlett Learning, LLC © Jones & Bartlett Learning, LLC NOT FOR SALE OR DISTRIBUTION NOT FOR SALE OR DISTRIBUTION © Jones & Bartlett Learning, LLC © Jones & Bartlett Learning, LLC NOT FOR SALE OR DISTRIBUTION NOT FOR SALE OR DISTRIBUTION A Flame loop. B Remove cap of tube. C Flame tip of tube. D Obtain bacteria from culture tube. © Jones & Bartlett Learning, LLC © Jones & Bartlett Learning, LLC NOT FOR SALE OR DISTRIBUTION NOT FOR SALE OR DISTRIBUTION © Jones & Bartlett Learning, LLC © Jones & Bartlett Learning, LLC NOT FOR SALE OR DISTRIBUTION NOT FOR SALE OR DISTRIBUTION © Jones & Bartlett Learning, LLC © Jones & Bartlett Learning, LLC E F Replace cap. NOTFlame FOR tip of SALE tube. OR DISTRIBUTION G PlaceNOT bacteria FOR on slide. SALE OR DISTRIBUTIONH Reflame loop. FIGURE 1 Important steps in the preparation of a bacterial smear. © Jones & Bartlett9. Air-dryLearning,the slide LLC until all the liquid evaporates.© Jones An & electric Bartlett warming Learning, tray LLC NOT FOR SALE ORmay DISTRIBUTION be used for this purpose. Caution shouldNOT FOR be taken SALE to avoid OR DISTRIBUTIONextreme heat because cell distortion and splattering may occur. 10. Heat-fix the smears by quickly passing the slide through the Bunsen burner flame three times (Figure 2). The heat should contact the underside © Jones & Bartlett Learning, LLC © Jones & Bartlett Learning, LLC NOT FOR SALE OR DISTRIBUTION NOT FOR SALE OR DISTRIBUTION © Jones & Bartlett Learning, LLC © Jones & Bartlett Learning, LLC NOT FOR SALE OR DISTRIBUTION NOT FOR SALE OR DISTRIBUTION FIGURE 2 © Jones & Bartlett Learning, LLC A slide is heat-fixed© Jones by passing & Bartlett it quickly over Learning, a flame LLC several times. NOT FOR SALE OR DISTRIBUTION NOT FOR SALE OR DISTRIBUTION © Jones & Bartlett Learning, LLC. NOT FOR SALE OR DISTRIBUTION.5054 © Jones & Bartlett Learning, LLC of the slide. This procedure© Jones 1) & killsBartlett any bacteria Learning, that LLCmay still be alive, NOT FOR SALE OR DISTRIBUTION2) facilitates stain penetration,NOT FOR and SALE 3) fixes OR cells DISTRIBUTION to the slide so that they do not wash off when stained. The slide is now ready to be stained. © Jones & Bartlett Learning, LLC © Jones & Bartlett Learning, LLC NOT FORB. SALEThe OR Simple DISTRIBUTION Stain Technique NOT FOR SALE OR DISTRIBUTION PURPOSE: to determine the The simple stain technique is a rapid and effective way of preparing a size, shape, and arrangement bacterial smear for viewing.

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