In the first of these reports (Wenrich, 1946), it was pointed out that the cultivation of intestinal flagellates was originally undertaken as an aid in the study of trichomonad morphology. Two additional objectives have developed during the course of the work: 1) to determine the length of time that various intestinal flagellates will survive in individual culture tubes if, when populations begin to decline, additional nutrients are supplied and water is added to maintain the quantity of fluid; and 2) to consider the correlation between the capacity to live under diverse cultural conditions and the ability to reach new hosts. The present account includes results obtained on flagellates from amphibians and reptiles up to the end of October, 1946. I am indebted to Mr. H. A. Walters for the opportunity to examine two pilot black snakes (Elaphe obsoleta) and a Mobile turtle (Pseudemys floridana mobilensis) ; to Dr. T. S. Hauschka for collecting specimens of the blue-spotted salamander (Ambystorna jeffersonianum) and the northern red salamander (Pseudotriton ruber) ; to Dr. R. M. Stabler for other amphibians; and to Miss Bernice Goldis, who, under the supervision of Dr. L. V. Heilbrunn, made determinations of pH and of freezing-point depressions. This study has been aided by a grant from the Research Fund of the University of Pennsylvania. The methods previously outlined have been employed. The chief basic fluids have been 1) Drbohlav's (1925) modified Ringer's fluid (R2) and 2) boiled pond water (W). Sometimes regular Ringer's (R1), with 0.8% NaC1, or various dilutions of it, have been used. The principal nutrients have been 1) gastric mucin (M), and 2) Difco Loeffler's dried blood serum (L), both commonly in a concentration of 0.2%. For initial inoculations these substances were dissolved in the fluids, but when added later they were frequently in the dry state, unless liquid was also to be added, in which case, they were dissolved, usually in distilled water. Additional nutrients employed will be referred to in the descriptions and tables; in the explanation of the latter the meanings of the other abbreviations may also be found. Longevity figures give the number of days that individual tubes remained positive. As in the previous paper, original cultures are indicated by a capital letter following a strain number. Subcultures are designated by a small letter after a transplant-generation number. For example, in the third line of Table 2, culture 1E/4a is the first tube (a) of the fourth subculture-generation from the fifth (E) tube among the original cultures from frog 1. Since the original cultures were inoculated from feces or intestinal contents, the bacterial flora of these cultures originated from the same source. The usual precautions were taken to prevent the entrance of organisms from the air.