Diagnostic Medical Parasitology. Lynne Shore Garcia

      Figure 3.15 Work flow diagram for fecal specimens. The total examination includes the direct mount, concentrate, and permanent stained smear (fresh specimen) or the concentrate and permanent stained smear (preserved specimens). doi:10.1128/9781555819002.ch3.f15

      Although an experienced microscopist can occasionally identify certain organisms on a wet preparation, most identifications should be considered tentative until confirmed by the permanent stained slide. The smaller protozoan organisms are frequently seen on the stained smear when they are easily missed with only the direct smear and concentration methods. For these reasons, the permanent stain is recommended for every stool sample submitted for a routine parasite examination. It is also important to remember that the fecal immunoassays for specific organisms have proven to be more sensitive than the routine or specialized stains for Giardia lamblia (G. duodenalis, G. intestinalis) or Cryptosporidium spp. (25, 26).

      There are a number of staining techniques available; selection of a particular method may depend on the degree of difficulty of the procedure and the amount of time necessary to complete the stain. The older classical method is the long Heidenhain iron hematoxylin method; however, for routine diagnostic work, most laboratories select one of the shorter procedures, such as the trichrome method or one of the modified methods involving iron hematoxylin. Other procedures are available (4, 6–8, 13, 17, 20, 24, 27, 30, 49), and some of them are presented here.

      Most problems encountered in the staining of protozoan trophozoites and cysts in fecal smears occur because the specimen is too old, the smears are too dense, the smears are allowed to dry before fixation, or fixation is inadequate. There is variability in fixation in that immature cysts fix more easily than mature cysts, and E. coli cysts require a longer fixation time than do those of other species. It is critical that adequate mixing occur between the fecal specimen and preservative (27–29, 31, 32).

      Preparation of Material for Staining

      Fresh Material

      1. When the specimen arrives, prepare two slides with applicator sticks or brushes and immediately (without drying) place them in Schaudinn’s fixative [(This approach is rarely used because the formulation contains mercury). Preserved stool collected in fecal fixatives (with or without PVA) can be smeared on a slide and allowed to air dry prior to staining.] Allow the slides to fix for a minimum of 30 min; overnight fixation is acceptable. The amount of fecal material smeared on the slide should be thin enough that newsprint can be read through the smear. Smears preserved in liquid Schaudinn’s fixative should be placed in 70% alcohol to remove the excess fixative prior to placement in iodine-alcohol (used for mercury-based fixatives).

      2. If the fresh specimen is liquid, place 3 or 4 drops of fixative (Schaudinn’s fixative to which has been added a plastic powder [PVA], which serves as an adhesive to “glue” the fecal material onto the slide) on the slide, mix several drops of fecal material with the PVA fixative, spread the mixture, and allow it to dry for several hours in a 37°C incubator or overnight at room temperature.

      3. Proceed with the trichrome staining procedure by placing the slides in iodine-alcohol.

      Preserved Material Containing PVA

      1. Stool specimens that are preserved in fixative (mercuric chloride, copper sulfate, or zinc sulfate bases) containing PVA should be allowed to fix for at least 30 min. Thoroughly mix the contents of the vial or bottle (fixative/stool/PVA specimen) with two applicator sticks.

      2. Pour some of the well-mixed fixative/stool/PVA mixture onto a paper towel, and allow it to stand for 3 min to absorb out the excess PVA. Do not eliminate this step.

      3. With an applicator stick (or brush), apply some of the stool material from the paper towel to two slides and allow them to dry for several hours in a 37°C incubator or overnight at room temperature.

      Note The fixative/stool/PVA mixture should be spread to the edges of the glass slide; this will cause the film to adhere to the slide during staining. It is also important to thoroughly dry the slides in order to prevent the material from washing off during staining.

      4. The dry slides may then be placed into iodine-alcohol. There is no need to give them a 70% alcohol rinse before placing them in the iodine-alcohol, because the PVA smears are already dry (unlike the wet smears coming out of Schaudinn’s fixative). The iodine-alcohol is used to remove the mercuric chloride from the slides before they are stained. When reviewing the trichrome staining procedure, you will note that this step is not required if the stool specimen is preserved in a copper sulfate or zinc sulfate-based preservative.

      NOTE Polyvinyl alcohol (PVA) is a plastic powder that is often added to fecal fixatives to help “glue” the stool material onto the glass slide. PVA is inert and has no fixing properties. Its main purpose is to cause the fecal material to adhere to the glass once the material is dry. HOWEVER, the Universal Fixatives do not require PVA or albumin to serve as adhesives.

      California State Department of Health Modification (1) for PVA-Preserved Material

      1. Thoroughly mix the fixative/stool/PVA mixture, and strain it through damp (with