Lectin blot studies on proteins of Myxobolus cerebralis, the causative agent of whirling disease

Knaus, Martin; El‐Matbouli, Mansour

doi:10.3354/dao065227

Cited by 8 publications

(10 citation statements)

References 48 publications

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“…Pre-esporogonic and extra-esporogonic stages of T. bryosalmonae were also stained by BSI-I at LM (Marín de Mateo et al 1996;Morris and Adams 2004), though only some vacuolar structures of P cell were scarcely labelled at TEM (Morris and Adams 2004). Using blot studies, Knaus and El-Matbouli (2005b) identified glycoproteins that contained carbohydrate motifs reactive with the same lectin in Myxobolus cerebralis stages as well.…”

Section: Discussionmentioning

confidence: 96%

Detection of carbohydrate terminals in the enteric parasite Enteromyxum scophthalmi (Myxozoa) and possible interactions with its fish host Psetta maxima

et al. 2008

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Section: Discussionmentioning

confidence: 96%

Detection of carbohydrate terminals in the enteric parasite Enteromyxum scophthalmi (Myxozoa) and possible interactions with its fish host Psetta maxima

et al. 2008

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“…Such terminal sugar re sidues are believed to play a paramount role in host− parasite interactions and may form a protective sheath for the parasites that helps them to evade host recognition (Hicks et al 2000, Theodoropoulos et al 2001. Therefore, some parasites, such as Trypanosoma cruzi (Buscaglia et al 2006), employ an antigen variation strategy through modification of N-and Oglycosides of glycoepitopes in their surface glycoproteins (Gagneux & Varki 1999, Knaus & El-Matbouli 2005. In fish, as in all vertebrates, the lectin pathway of the complement system is an ancient first line defense mechanism of the innate immune system that relies on recognition of pathogen-associated glycan epitopes (Sunyer & Lambris 1998, Nakao et al 2006, Kania et al 2010.…”

Section: Introductionmentioning

confidence: 99%

“…In fish, as in all vertebrates, the lectin pathway of the complement system is an ancient first line defense mechanism of the innate immune system that relies on recognition of pathogen-associated glycan epitopes (Sunyer & Lambris 1998, Nakao et al 2006, Kania et al 2010. In previous studies, the glycoproteins of some piscine parasites have been studied by lectin blotting (Feng & Woo 1998b, Kim et al 1999, Muñoz et al 2000a, Knaus & El-Matbouli 2005.…”

Section: Introductionmentioning

confidence: 99%

“…Another approach to studying the antigenicity of myxozoans is the use of polyclonal antibodies (Pabs) (Bartholomew et al 1989, Saulnier & deKinkelin 1996, Muñoz et al 1999b, 2000a, Lu et al 2002, Knaus & El-Matbouli 2005, Zhang et al 2010). In the present study, the antigenic glycoproteins of Enteromyxum leei were analysed using 2 Pabs; one raised against E. leei and another raised against the polar filament of Myxobolus pendula (Ringuette et al 2011).…”

Section: Introductionmentioning

confidence: 99%

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Antigenic characterization of Enteromyxum leei (Myxozoa: Myxosporea)

Estensoro¹,

Álvarez-Pellitero²,

Sitjà‐Bobadilla³

2013

Dis. Aquat. Org.

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Enteromyxum leei, an intestinal myxozoan parasite affecting a wide range of fish, was partially purified, and the immunogenic composition of its glycoproteins as well as the proteolytic activity were studied. Parasite extracts, mainly containing spores, were separated by SDS-PAGE, and thereafter, immunoblots were carried out with a polyclonal antiserum (Pab) raised against E. leei. Periodic acid/Schiff staining of gels, periodate- and Proteinase K-treated Western blots and Lectin blots were performed to analyse the terminal carbohydrate composition of the parasite's antigens. Additionally, the cross-reaction of the parasite extracts with a Pab raised against the polar filament of the myxozoan Myxobolus pendula was studied. Both Pabs detected proteic epitopes on antigenic proteins and glycoproteins of E. leei, ranging between 15 and 280 kDa. In particular, 2 glycoproteic bands (15 and 165 kDa), immunoreactive to both Pabs and with glucose and mannose moieties, could correspond to common antigens shared among myxozoans. The 165 kDa band also presented galactose, N-acetyl-galactosamine and N-acetyl-glucosamine, pointing to its possible origin on chitin-built spore valves and to its possible involvement in host-parasite interactions. The molecular weight of the 15 kDa glycoproteic antigen matches that of minicollagen, a cnidarian-specific protein of nematocysts with a myxozoan homologue. Several proteases with apparent molecular weights ranging between 43 and 245 kDa were found in zymographies of E. leei extracts, and these may have a potential role in the parasite's pathogenesis. This is a useful approach for further studies to detect targets for antiparasitic therapy.

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“…However, this approach can be time-and laborconsuming, and detection and identification is mainly based on the mature spore stages, with the early parasite stages likely to be neglected (Grabner et al 2012, Mahony et al 2015. Immunological methods based on antibodies or lectins (Knaus & El-Matbouli 2005, Estensoro et al 2013) have also been developed. Nevertheless, these methods are generally restricted by cross-reactivity between different species (Lu et al 2002, Estensoro et al 2014, Jia et al 2016.…”

Section: Introductionmentioning

confidence: 99%

Development of a multiplex PCR method for the simultaneous detection of four myxosporeans infecting gibel carp Carassius auratus gibelio

Li¹,

Zhai²,

Gu³

et al. 2017

Dis. Aquat. Org.

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Gibel carp Carassius auratus gibelio (Bloch), a commercially important freshwatercultured fish in China, is threatened by myxosporeans, particularly Thelohanellus wuhanensis, Myxobolus honghuensis, M. wulii and M. turpisrotundus. Here, we developed a multiplex PCR assay for simultaneous detection of these 4 myxosporeans. The specific primers for each species were designed based on the 28S rDNA gene of T. wuhanensis, the ITS-5.8S rDNA of M. honghuensis and M. wulii, and the 18S rDNA gene of M. turpisrotundus. Specificity testing confirmed that the 4 primer sets have no cross-reactivity with other related myxosporean species tested. Detection limits of the multiplex PCR assay were 0.2, 0.3, 3.1 and 3.8 spores for T. wuhanensis, M. honghuensis, M. wulii and M. turpisrotundus, respectively. Following screening of 104 field samples, the analytical sensitivity of the present multiplex PCR assay was found to be similar to the sensitivity obtained by the singleplex PCR assays and was higher than that of microscopic examination. Moreover, Kappa analysis showed a strong agreement between the results of the singleplex and multiplex PCR assays, indicating that the developed multiplex PCR assay was an efficient approach for the diagnosis of the 4 myxosporeans infecting gibel carp. KEY WORDS: Multiplex PCR · Molecular detection · Myxosporeans · Gibel carp · rDNA Resale or republication not permitted without written consent of the publisherDis Aquat Org 124: [31][32][33][34][35][36][37][38][39] 2017 forms plasmodia in the skin of the host and is responsible for chronic mortality and poor growth (Liu et al. 2014b). Minimizing the severe negative impact of myxosporidiosis on commercially important gibel carp is considered a priority in China. Early and accurate detection of myxosporeans could help fish farmers to carry out prompt drug therapy and minimize the likelihood of a myxo sporidiosis outbreak (Jia et al. 2015). Therefore, a simple and efficient assay for detection of myxo sporean pathogens is needed.Microscopic examination of squash preparations or histological sections is the most direct and commonly used method to detect and distinguish myxosporean parasites (St-Hilaire et al. 1997, Kelley et al. 2004). However, this approach can be time-and laborconsuming, and detection and identification is mainly based on the mature spore stages, with the early parasite stages likely to be neglected (Grabner et al. 2012, Mahony et al. 2015. Immunological methods based on antibodies or lectins (Knaus & El-Matbouli 2005, Estensoro et al. 2013) have also been developed. Nevertheless, these methods are generally restricted by cross-reactivity between different species (Lu et al. 2002, Estensoro et al. 2014, Jia et al. 2016. In recent years, PCR-based molecular detection and identification with higher sensitivity, specificity and rapidity has been utilised widely in myxo sporean examination (Qureshi et al. 2002, Cavender et al. 2004, Clark 2006, Grabner et al. 2012, Jeon et al. 2014. Given the multiple copies and moderate i...

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Lectin blot studies on proteins of Myxobolus cerebralis, the causative agent of whirling disease

Cited by 8 publications

References 48 publications

Detection of carbohydrate terminals in the enteric parasite Enteromyxum scophthalmi (Myxozoa) and possible interactions with its fish host Psetta maxima

Detection of carbohydrate terminals in the enteric parasite Enteromyxum scophthalmi (Myxozoa) and possible interactions with its fish host Psetta maxima

Antigenic characterization of Enteromyxum leei (Myxozoa: Myxosporea)

Development of a multiplex PCR method for the simultaneous detection of four myxosporeans infecting gibel carp Carassius auratus gibelio

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