Bile Acids Enhance Invasiveness of
            <i>Cryptosporidium</i>
            spp. into Cultured Cells

Feng, Hanping; Nie, Weijia; Sheoran, Abhineet S.; Zhang, Quanshun; Tzipori, Saul

doi:10.1128/iai.00169-06

Cited by 28 publications

(35 citation statements)

References 32 publications

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“…Excystation in the presence of both bile salt and Caco2 cells, however, was significantly better than in samples containing cells only. Bile salts may have a separate major role in parasite infection by activating sporozoite gliding required for host cell invasion (8).…”

Section: Discussionmentioning

confidence: 99%

“…Both raised temperature and acidic conditions have been demonstrated to increase the permeability of the oocyst wall to small molecules (20). It has been established that bile salts increase the rate of excystation, and a study reported that, in addition, sodium deoxycholate improved the invasiveness of sporozoites for epithelial cells (8). Increased parasite protease activity during excystation has been described, and sporozoite release was hindered by protease inhibitors (9).…”

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confidence: 99%

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The Terminal Sialic Acid of Glycoconjugates on the Surface of Intestinal Epithelial Cells Activates Excystation of Cryptosporidium parvum

2008

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The apicomplexan Cryptosporidium parvum reproduces in the intestinal epithelial cells of many mammalian species and is an agent of the important diarrheal disease cryptosporidiosis. Infection is transmitted fecalorally by oocysts that pass through the stomach and excystation occurs in the intestine, releasing four invasive sporozoites. Some factors involved in inducing excystation have been identified, but the role of the enterocyte is not known. The present study showed that excystation was accelerated in the presence of the three enterocyte cell lines Caco2, HCT8, and CMT93. Epithelial cell lines derived from other organs, including the stomach, had no effect on excystation. No evidence was obtained that factors secreted from enterocytes induced excystation, but an enterocyte membrane preparation promoted sporozoite release. In addition, modification of the enterocyte surface by trypsin digestion or paraformaldehyde fixation abrogated the ability to enhance excystation. Importantly, the level of excystation in the presence of enterocytes decreased after treatment with either sialidase/neuraminidase to deplete surface terminal sialic acid or with lectins that specifically bind to sialic acid. Furthermore, the addition of sialic acid to oocysts in the absence of cells increased the level of excystation. These results suggest that sialic acid on the surface of enterocytes may provide an important local signal for the excystation of C. parvum sporozoites.

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Section: Discussionmentioning

confidence: 99%

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confidence: 99%

The Terminal Sialic Acid of Glycoconjugates on the Surface of Intestinal Epithelial Cells Activates Excystation of Cryptosporidium parvum

2008

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“…Subconfluent HCT-8 monolayers seeded in T75 flasks were infected with C. parvum oocysts at a 1:4 oocyst/host cell ratio and incubated for 24 h. This time point was chosen because at later time points monolayer perturbance increases. Taurocholic acid at a concentration of 0.05% was added with the oocysts to promote infection (11). After incubation, cell monolayers were recovered by treatment with Accutase (Innovative Cell Technologies, Inc.) and immunofluorescently labeled as described previously (31), except that polyclonal rabbit antibody specific for C. parvum sporozoites and oocysts was used as the primary antibody and the host cell membrane was not permeabilized.…”

Section: Methodsmentioning

confidence: 99%

Cell Sorting-Assisted Microarray Profiling of Host Cell Response to Cryptosporidium parvum Infection

2010

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To study the transcriptional response of mammalian cells to infection with the intracellular apicomplexan parasite Cryptosporidium parvum, infected and uninfected cells were recovered from C. parvum-infected cell monolayers. This approach, which contrasts with a more conventional experimental design that compares infected to uninfected cell monolayers, enabled the identification of functional categories of genes that are differentially transcribed as a direct consequence of the presence of intracellular parasites. Among several categories of upregulated genes, glycoprotein metabolism was significantly overrepresented. To investigate whether these transcriptional changes affected the composition of the surface of infected cells, cells were probed with fluorescently labeled lectins. Among a panel of seven lectins, soybean agglutinin, which recognizes N-acetyl-D-galactosamine, generated the largest difference in fluorescence between infected and uninfected cells. The origin of the fluorescent signal emitted by infected cells was further investigated and attributed to the overexpression of glycoprotein on the surface of infected cells, as well as the presence of glycoprotein located in the proximity of intracellular parasites.Cryptosporidium parvum, an apicomplexan protozoan species, infects the intestine and sometimes the respiratory tract and bile duct of various mammalian hosts. In immunocompetent humans the infection causes self-limited diarrhea, but in immunocompromised individuals, primarily those with AIDS, the infection can become chronic and potentially cause lifethreatening syndromes (5). Infection with Cryptosporidium parasites occurs when food or water contaminated with oocysts is ingested, or possibly through the inhalation of oocysts. After entering the gastrointestinal tract of the host, four sporozoites released from the oocyst seek to invade the intestinal epithelial cells, where they multiply as meronts.Global gene expression profiles in cell monolayers infected with C. parvum have been studied using microarrays (3,8,20). These studies found that genes belonging to the cell proliferation, apoptosis, signal transduction, and transcription categories are overrepresented among significantly regulated genes (8,20,39). The overexpression of the osteoprotegerin gene in host cells after infection also was reported (3).Published microarray studies of C. parvum-infected cells are based on RNA extracted from cells in culture. The development of this parasite in culture is restricted in time, and the completion of the life cycle is only rarely observed (14, 32). High oocyst doses and long incubation times do not increase the proportion of infected cells (36) and may instead lead to the extensive perturbation of the monolayer caused primarily by apoptosis and mitosis (19,21,34,38). Discerning which transcriptional changes occur directly in response to the infection, and which result from the perturbance of the monolayer (13, 36), is difficult. To eliminate the effect of partial infection and monolayer perturba...

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“…However, progress in research on these organisms has been hampered by the limitations of current experimental models (6). Because animal models are suboptimal for some human infections, human colonic cell lines have been used as an alternative to study intestinal pathogens (7,8). The utility of cell lines is limited by the fact they are not derived from the small intestine and are transformed.…”

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confidence: 99%

Human Primary Intestinal Epithelial Cells as an Improved In Vitro Model for Cryptosporidium parvum Infection

et al. 2013

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The study of human intestinal pathogens has been limited by the lack of methods for the long-term culture of primary human intestinal epithelial cells (PECs). The development of infection models with PECs would allow a better understanding of hostparasite interactions. The objective of this study was to develop a novel method for prolonged in vitro cultivation of PECs that can be used to study Cryptosporidium infection. We isolated intact crypts from human intestines removed during weight loss surgery. The fragments of intestinal layers were cultivated with culture medium supplemented with growth factors and antiapoptotic molecules. After 7 days, the PECs formed self-regenerating cell clusters, forming villi that resemble intestinal epithelium. The PECs proliferated and remained viable for at least 60 days. The cells expressed markers for intestinal stem cells, epithelial cells, and mature enterocytes. The PECs were infected with Cryptosporidium. In contrast to older models in which parasite numbers decay, the burden of parasites increased for >120 h. In summary, we describe here a novel method for the cultivation of self-regenerating human epithelial cells from small intestinal crypts, which contain both intestinal stem cells and mature villus cells. We present data that suggest these cells support Cryptosporidium better than existing cell lines. PECs should provide an improved tool for studying host-parasite interactions involving Cryptosporidium and other intestinal pathogens.

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Bile Acids Enhance Invasiveness of Cryptosporidium spp. into Cultured Cells

Cited by 28 publications

References 32 publications

The Terminal Sialic Acid of Glycoconjugates on the Surface of Intestinal Epithelial Cells Activates Excystation of Cryptosporidium parvum

The Terminal Sialic Acid of Glycoconjugates on the Surface of Intestinal Epithelial Cells Activates Excystation of Cryptosporidium parvum

Cell Sorting-Assisted Microarray Profiling of Host Cell Response to Cryptosporidium parvum Infection

Human Primary Intestinal Epithelial Cells as an Improved In Vitro Model for Cryptosporidium parvum Infection

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