Development of improved PCR to prevent false positives and false negatives in the detection of<i>Tetracapsula bryosalmonae</i>, the causative agent of proliferative kidney disease

Morris, D C; Morris, David J.; Adams, Alexandra

doi:10.1046/j.1365-2761.2002.00398.x

Cited by 21 publications

(24 citation statements)

References 22 publications

Supporting

Mentioning

Contrasting

Order By: Relevance

“…Although very faint, yet consistent products were attained at an estimated 0.01 spore, human error caused by the inability to visualise such a weak signal is likely to result in a false negative outcome. Sensitivity for this diagnostic assay is similar to previous myxozoan single-round PCR based tests developed to date (Kent et al 1998, Palenzuela et al 1999, Morris et al 2002 and is more sensitive than current diagnostic methods. Accuracy in diagnosis is also improved by the ability to process whole fish, whole brains and spinal cords, whereas techniques such as microscopic examination of 5 µm sections only examines a portion of the targeted tissue introducing greater probability of error.…”

Section: Discussionsupporting

confidence: 73%

“…Fourteen adult blue throat wrasse and 20 striped trumpeter from each life stage at 23, 44, 77 and 136 dph were tested for parasites using wet squash preparations (Wet), H&E stained 5 µm sections (H&E) and PCR. Positive and negative infections are shown as + and -respectively and the percentage of positive infections are calculated at the bottom of each column for the blue throat wrasse model 1998, Palenzuela et al 1999, Morris et al 2002, Yokoyama et al 2000. The single-round PCR test was able to specifically amplify a fragment of the SSU rDNA from Kudoa neurophila and strong amplicons were always visualised from fish known to harbour the parasite infection at the terminal stage as determined by traditional histology.…”

Section: Discussionmentioning

confidence: 99%

“…The test is also designed to utilise commercially available molecular, easy to operate biology kits that have been shown here to be effective, efficient and reliable when used in the field situation. Myxozoan detection research has determined similar outcomes using the PCR approach to diagnosis and health management for both wild fishery management and aquaculture worldwide (Saulnier & de Kinkelin 1997, Andree et al 1998, Kent et al 1998, Palenzuela et al 1999, Morris et al 2002, Yokoyama et al 2000. The single-round PCR test was able to specifically amplify a fragment of the SSU rDNA from Kudoa neurophila and strong amplicons were always visualised from fish known to harbour the parasite infection at the terminal stage as determined by traditional histology.…”

mentioning

confidence: 92%

“…A very sensitive and specific DNA-based diagnostic test using standard polymerase chain reaction (PCR) molecular technology is a management tool capable of detecting early developmental stages of the parasite or very light but mature infections in the fish host. The ability of PCR to perform this function is particularly useful as it can detect sub-clinical myxozoan infections much earlier than routine histology (Saulnier & de Kinkelin 1997, Andree et al 1998, Kent et al 1998, Palenzeula et al 1999, Yokoyama et al 2000, Morris et al 2002. In the case of K. neurophila, traditional techniques such as light microscope examination of stained sections and wet squash preparations are only effective in detecting the terminal spore forming stage and, in rare instances, presporogonic plasmodial stages of the disease.…”

Section: Introductionmentioning

confidence: 99%

See 3 more Smart Citations

Diagnostic polymerase chain reaction assay to detect Kudoa neurophila (Myxozoa: Multivalvulida) in a marine finfish hatchery

Grossel¹,

Handlinger²,

Battaglene³

et al. 2005

Dis. Aquat. Org.

View full text Add to dashboard Cite

A single-round polymerase chain reaction (PCR) diagnostic assay was developed from a small subunit ribosomal DNA (SSU rDNA) gene sequence to detect the myxozoan parasite Kudoa neurophila, the causative agent of myxozoan disease in the hatchery reared marine finfish, striped trumpeter Latris lineata (Forster). The assay was developed for use as a disease control management tool in a hatchery system specifically designed to research and produce marine finfish such as striped trumpeter juveniles for aquaculture. The assay is sufficiently species specific and sensitive enough to detect a small fragment of the parasite's SSU rDNA. At the lower limits of detection, the test is consistently positive to an estimated 0.1 spore or 60 fg of parasite DNA per 25 µl PCR reaction in serial dilution and positive to an estimated 0.1 spore in 25 mg of infected fish CNS tissue (4 spores g -1 ). Specifically, the test is capable of detecting early stages of the life cycle within the fish host and consequently diagnosing an infection not normally detected using traditional histological techniques. The test is also effective for screening water supplies and prey species cultures throughout the hatchery system to determine bio-security efficacy, to assist in identification of an alternate or other primary fish host, to indicate the location of potential disease reservoirs, and to enable a targeted approach to disease prevention. KEY WORDS: Aquaculture · Myxozoa · Kudoa neurophila · PCR · Striped trumpeter Resale or republication not permitted without written consent of the publisherDis Aquat Org 64: [141][142][143][144][145][146][147][148][149] 2005 respectively (Wolf & Markiw 1984). An invertebrate or alternative host for K. neurophila responsible for releasing the infective actinosporean stage of the parasite has not yet been discovered, although juvenile fish are believed to become infected during larval stages and develop nervous aberrations suggestive of a disease of the CNS around 70 d post hatch (dph). Mature spores of K. neurophila representing the terminal life cycle stage within the fish host can first be detected with a high prevalence of infection (100% in surviving fish) from approximately 100 dph (Grossel et al. 2002). This developmental pattern is similar to other closely related marine Myxozoa such as Kudoa thyrsites in netpen-reared Atlantic salmon (Moran et al. 1999). K. neurophila has been recognised as a significant disease restricting striped trumpeter culture assessment. The disease directly inhibits the production of sufficient quantities of viable juvenile fish required to test large-scale marine aquaculture.Pentavalvid forms of Kudoa were previously morphologically distinguishable as species belonging to the genus Pentacapsula by having 5 shell valves and 5 polar capsules (Naidenova & Zaika 1970, Lom & Dykova 1992 with only 4 species discovered to date (Naidenova & Zaika 1970, Cheung et al. 1983, Kovaleva & Gaevskaya 1984, Grossel et al. 2003. However, comparative small subunit ribosomal DNA (SSU...

show abstract

Section: Discussionsupporting

confidence: 73%

Section: Discussionmentioning

confidence: 99%

mentioning

confidence: 92%

Section: Introductionmentioning

confidence: 99%

See 2 more Smart Citations

Diagnostic polymerase chain reaction assay to detect Kudoa neurophila (Myxozoa: Multivalvulida) in a marine finfish hatchery

Grossel¹,

Handlinger²,

Battaglene³

et al. 2005

Dis. Aquat. Org.

View full text Add to dashboard Cite

show abstract

“…The yield was determined by spectrophotometry using the NanoDrop photometer (NanoDrop Technologies). PCR was performed according to the protocol by Morris et al (2002), with some modifications. The primer pair PKX3F (CTA AGT ACA TAC TTC GGT AGA) and PKX4R (CCG TTA CAA CCT TGT TAG GAA), described by Kent et al (1998), was used.…”

Section: Pcr For Detection Of Tetracapsuloides Bryosalmonae Dna In Kimentioning

confidence: 99%

Complex interaction between proliferative kidney disease, water temperature and concurrent nematode infection in brown trout

Schmidt‐Posthaus¹,

Steiner²,

Müller³

et al. 2013

Dis. Aquat. Org.

View full text Add to dashboard Cite

Proliferative kidney disease (PKD) is a temperature-dependent disease caused by the myxozoan Tetracapsuloides bryosalmonae. It is an emerging threat to wild brown trout Salmo trutta fario populations in Switzerland. Here we examined (1) how PKD prevalence and pathology in young-of-the-year (YOY) brown trout relate to water temperature, (2) whether wild brown trout can completely recover from T. bryosalmonae-induced renal lesions and eliminate T. bryosalmonae over the winter months, and (3) whether this rate and/or extent of the recovery is influenced by concurrent infection. A longitudinal field study on a wild brown trout cohort was conducted over 16 mo. YOY and age 1+ fish were sampled from 7 different field sites with various temperature regimes, and monitored for infection with T. bryosalmonae and the nematode Raphidascaris acus. T. bryosamonae was detectable in brown trout YOY from all sampling sites, with similar renal pathology, independent of water temperature. During winter months, recovery was mainly influenced by the presence or absence of concurrent infection with R. acus larvae. While brown trout without R. acus regenerated completely, concurrently infected brown trout showed incomplete recovery, with chronic renal lesions and incomplete translocation of T. bryosalmonae from the renal interstitium into the tubular lumen. Water temperature seemed to influence complete excretion of T. bryosalmonae, with spores remaining in trout from summer-warm rivers, but absent in trout from summer-cool rivers. In the following summer months, we found PKD infections in 1+ brown trout from all investigated river sites. The pathological lesions indicated a reinfection rather than a proliferation of remaining T. bryosalmonae. However, disease prevalence in 1+ trout was lower than in YOY.

show abstract

Improved Conventional PCR Assay for Detecting Tetracapsuloides bryosalmonae DNA in Fish Tissues

et al. 2018

View full text Add to dashboard Cite

Conventional PCR is an established method to detect Tetracapsuloides bryosalmonaeDNA in fish tissues and to confirm diagnosis of proliferative kidney disease (PKD) caused by T. bryosalmonae. However, the commonly used PKX5f-6r primers were designed with the intention of obtaining sequence information and are suboptimal for determining parasite DNA presence. A new PCR assay to detect T. bryosalmonae 18s rDNA, PKX18s1266f-1426r, is presented that demonstrates specificity, repeatability, and enhanced sensitivity over the PKX5f-6r assay. The limit of detection of the PKX18s1266f-1426r assay at 95% confidence was 100 template copies, and the new primers detected parasite DNA more consistently at template concentrations below 100 copies than did PKX5f-6r. The PKX18s1266f-1426r also achieved 100% detection at sample DNA concentrations one order of magnitude lower than PKX5f-6r. Out of 127 salmonid fish with unknown T. bryosalmonae infection status, PKX5f-6r detected 35 positive samples, while the new assay detected 43. The discrepancy in T. bryosalmonae detection between the two primer sets may be attributed to several differences between the assays, including oligonucleotide melting temperatures, the use of a touchdown PCR thermal cycle, and amplicon length.

show abstract

Development of improved PCR to prevent false positives and false negatives in the detection ofTetracapsula bryosalmonae, the causative agent of proliferative kidney disease

Cited by 21 publications

References 22 publications

Diagnostic polymerase chain reaction assay to detect Kudoa neurophila (Myxozoa: Multivalvulida) in a marine finfish hatchery

Diagnostic polymerase chain reaction assay to detect Kudoa neurophila (Myxozoa: Multivalvulida) in a marine finfish hatchery

Complex interaction between proliferative kidney disease, water temperature and concurrent nematode infection in brown trout

Improved Conventional PCR Assay for Detecting Tetracapsuloides bryosalmonae DNA in Fish Tissues

Contact Info

Product

Resources

About