Marilyn M. Marshall scite author profile

In vitro cell cultures were compared to neonatal mice for measuring the infectivity of five genotype 2 isolates of Cryptosporidium parvum. Oocyst doses were enumerated by flow cytometry and delivered to animals and cell monolayers by using standardized procedures. Each dose of oocysts was inoculated into up to nine replicates of 9 to 12 mice or 6 to 10 cell culture wells. Infections were detected by hematoxylin and eosin staining in CD-1 mice, by reverse transcriptase PCR in HCT-8 and Caco-2 cells, and by immunofluorescence microscopy in Madin-Darby canine kidney (MDCK) cells. Infectivity was expressed as a logistic transformation of the proportion of animals or cell culture wells that developed infection at each dose. In most instances, the slopes of the dose-response curves were not significantly different when we compared the infectivity models for each isolate. The 50% infective doses for the different isolates varied depending on the method of calculation but were in the range from 16 to 347 oocysts for CD-1 mice and in the ranges from 27 to 106, 31 to 629, and 13 to 18 oocysts for HCT-8, Caco-2, and MDCK cells, respectively. The average standard deviations for the percentages of infectivity for all replicates of all isolates were 13.9, 11.5, 13.2, and 10.7% for CD-1 mice, HCT-8 cells, Caco-2 cells, and MDCK cells, respectively, demonstrating that the levels of variability were similar in all assays. There was a good correlation between the average infectivity for HCT-8 cells and the results for CD-1 mice across all isolates for untreated oocysts (r ‫؍‬ 0.85, n ‫؍‬ 25) and for oocysts exposed to ozone and UV light (r ‫؍‬ 0.89, n ‫؍‬ 29). This study demonstrated that in vitro cell culture was equivalent to the "gold standard," mouse infectivity, for measuring the infectivity of C. parvum and should therefore be considered a practical and accurate alternative for assessing oocyst infectivity and inactivation. However, the high levels of variability displayed by all assays indicated that infectivity and disinfection experiments should be limited to discerning relatively large differences.

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Waterborne protozoan pathogens.

Marshall

Naumovitz

Ortega

et al. 1997

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Using UV to inactivate Cryptosporidium

Clancy¹,

Bukhari²,

Hargy³

et al. 2000

Journal AWWA

150

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Even extremely low dosages of ultraviolet light can be highly effective for inactivating Cryptosporidium oocysts.Recent studies have shown that Cryptosporidium parvum oocysts demonstrate high susceptibility to low dosages of medium‐pressure ultraviolet (UV) light. These investigations have raised several questions, which include determination of minimum medium‐pressure UV dosages necessary to inactivate C. parvum oocysts, elucidation of differences (if any) between medium‐ and low‐pressure UV light for inactivating C. parvum oocysts, and evaluation of medium‐pressure UV effectiveness in inactivating oocysts suspended in poorer quality water. To compare low‐ and medium‐pressure UV, the authors exposed oocysts suspended in deionized water to UV delivered by either medium‐ or low‐pressure UV lamps at bench scale using a collimated beam apparatus. The applied UV dosages ranged from 3 to 33 mJ/cm2, and oocyst inactivation was assessed using the neonatal mouse infectivity assay. At 3 mJ/cm2, medium‐pressure UV showed a 3.4‐log inactivation of oocysts, and low‐pressure UV showed a 3.0‐log inactivation, demonstrating medium‐ and low‐pressure UV did not differ significantly in inactivating C. parvum oocysts.

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Waterborne Protozoan Pathogens

et al. 1998

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Species-Specific, Nested PCR-Restriction Fragment Length Polymorphism Detection of Single Cryptosporidium parvum Oocysts

Sturbaum

Reed

Hoover

et al. 2001

Appl Environ Microbiol

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Concurrent with recent advances seen with Cryptosporidium parvum detection in both treated and untreated water is the need to properly evaluate these advances. A micromanipulation method by which known numbers of C. parvum oocysts, even a single oocyst, can be delivered to a test matrix for detection sensitivity is presented. Using newly developed nested PCR-restriction fragment length polymorphism primers, PCR sensitivity was evaluated with 1, 2, 3, 4, 5, 7, or 10 oocysts. PCR detection rates (50 samples for each number of oocysts) ranged from 38% for single oocysts to 92% for 5 oocysts, while 10 oocysts were needed to achieve 100% detection. The nested PCR conditions amplified products from C. parvum, Cryptosporidium baileyi, and Cryptosporidium serpentis but no other Cryptosporidium sp. or protozoan tested. Restriction enzyme digestion with VspI distinguished between C. parvum genotypes 1 and 2. Restriction enzyme digestion with DraII distinguished C. parvum from C. baileyi and C. serpentis. Use of known numbers of whole oocysts encompasses the difficulty of liberating DNA from the oocyst and eliminates the standard deviation inherent within a dilution series. To our knowledge this is the first report in which singly isolated C. parvum oocysts were used to evaluate PCR sensitivity. This achievement illustrates that PCR amplification of a single oocyst is feasible, yet sensitivity remains an issue, thereby illustrating the difficulty of dealing with low oocyst numbers when working with environmental water samples.

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Comparison of Cryptosporidium parvum Viability and Infectivity Assays following Ozone Treatment of Oocysts

Bukhari¹,

Marshall

Korich

et al. 2000

Appl Environ Microbiol

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Several in vitro surrogates have been developed as convenient, user-friendly alternatives to mouse infectivity assays for determining the viability of Cryptosporidium parvum oocysts. Such viability assays have been used increasingly to determine oocyst inactivation following treatment with chemical, physical, or environmental stresses. Defining the relationship between in vitro viability assays and oocyst infectivity in susceptible hosts is critical for determining the significance of existing oocyst inactivation data for these in vitro assays and their suitability in future studies. In this study, four viability assays were compared with mouse infectivity assays, using neonatal CD-1 mice. Studies were conducted in the United States and United Kingdom using fresh (<1 month) or environmentally aged (3 months at 4°C) oocysts, which were partially inactivated by ozonation before viability and/or infectivity analyses. High levels of variability were noted within and between the viability and infectivity assays in the U.S. and United Kingdom studies despite rigorous control over oocyst conditions and disinfection experiments. Based on the viability analysis of oocyst subsamples from each ozonation experiment, SYTO-59 assays demonstrated minimal change in oocyst viability, whereas 4,6-diamidino-2-phenylindole-propidium iodide assays, in vitro excystation, and SYTO-9 assays showed a marginal reduction in oocyst viability. In contrast, the neonatal mouse infectivity assay demonstrated significantly higher levels of oocyst inactivation in the U.S. and United Kingdom experiments. These comparisons illustrate that four in vitro viability assays cannot be used to reliably predict oocyst inactivation following treatment with low levels of ozone. Neonatal mouse infectivity assays should continue to be regarded as a "gold standard" until suitable alternative viability surrogates are identified for disinfection studies.

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UV light inactivation of Cryptosporidium oocysts

Clancy¹,

Hargy²,

Marshall³

et al. 1998

Journal AWWA

115

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Animal infectivity studies demonstrate the efficacy of pulsed and advanced UV in inactivating Cryptosporidium oocysts. Cryptosporidium parvum oocysts are highly resistant to conventional chlorine‐based disinfectants. The authors tested two innovative electrotechnologies that use ultraviolet (UV) light and found that both pulsed UV and advanced UV inactivated Cryptosporidium oocysts. The advanced UV system achieved >4‐log inactivation as determined in animal infectivity studies using the neonatal mouse model. With the pulsed UV system, oocyst inactivation was also noted in the process control (non‐UV‐exposed oocysts), suggesting that some oocyst inactivation may have occurred independently of UV exposure. Irrespective of this, both technologies appear to be effective and novel ways to treat drinking water and to provide an additional significant barrier that helps protect public health.

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Irreversible UV Inactivation of Cryptosporidium spp. Despite the Presence of UV Repair Genes¹

Rochelle¹,

Fallar²,

Marshall

et al. 2004

J Eukaryotic Microbiology

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Ultraviolet light is being considered as a disinfectant by the water industry because it appears to be very effective for inactivating pathogens, including Cryptosporidium parvum. However, many organisms have mechanisms for repairing ultraviolet light-induced DNA damage, which may limit the utility of this disinfection technology. Inactivation of C. parvum was assessed by measuring infectivity in cells of the human ileocecal adenocarcinoma HCT-8 cell line, with an assay targeting a heat shock protein gene and using a reverse transcriptase polymerase chain reaction to detect infections. Oocysts of five different isolates displayed similar sensitivity to ultraviolet light. An average dosage of 7.6 mJ/cm2 resulted in 99.9% inactivation, providing the first evidence that multiple isolates of C. parvum are equally sensitive to ultraviolet disinfection. Irradiated oocysts were unable to regain pre-irradiation levels of infectivity, following exposure to a broad array of potential repair conditions, such as prolonged incubation, pre-infection excystation triggers, and post-ultraviolet holding periods. A combination of data-mining and sequencing was used to identify genes for all of the major components of a nucleotide excision repair complex in C. parvum and Cryptosporidium hominis. The average similarity between the two organisms for the various genes was 96.4% (range, 92-98%). Thus, while Cryptosporidum spp. may have the potential to repair ultraviolet light-induced damage, oocyst reactivation will not occur under the standard conditions used for storage and distribution of treated drinking water.

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