2. Methods2.1. Study site and sampl

2. Methods

2.1. Study site and sample

2.2. Test media and indicators

All samples were purchased in the morning and transported in an insulated bag in an air-conditioned vehicle, generally within 2 h of collection, to the Council for Scientific and Industrial Research Water Research Institute laboratory in Accra to be processed during the same day. Using American Public Health Association standards, we analyzed sachets for total coliforms (TC), fecal coliforms (FC), Escherichia coli (EC), and P. aeruginosa (PA) all in colony forming units (CFU) per 100 mL by using the membrane filtration method, and for total heterotrophic bacteria (THB) in CFU/mL by using the pour plate method (Rice, Baird, Eaton, & Clesceri, 2012). The full methods for TC, FC, EC, and THB are replicated from a prior study and described in detail elsewhere (Stoler et al., 2014). In preparing our sterile petri plates, we used the culture media MFC agar (Himedia) for FC, Hicrome Coliform agar (Fluka) for TC and EC, and Cetrimide agar base (Himedia) for PA prepared according to the manufacturer's instructions, and after incubation, colonies were counted using a colony counter. On MFC agar, blue colonies were recorded as FC. On Hicrome Coliform agar, dark-blue-to-violet colonies were recorded as EC, and all pink, salmon, red, and dark blue colonies were recorded as TC. On Cetrimide agar, blue green colonies exhibiting florescence under ultraviolet light (wavelength 250 nm) were presumed and recorded as PA. Plate readings of PA were subject to standard limitations noted on the manufacturer's technical data sheet (HiMedia, 2011) and common to most Cetri mide products.