The design of internal standard for mycobiome analysis of
clinical samples

a 2023

The design of internal standard for mycobiome analysis of clinical samples

FARNÍKOVÁ, Simona, Kateřina VYKLICKÁ, Petra BRENEROVÁ and Petra BOŘILOVÁ LINHARTOVÁ

Basic information

Original name

The design of internal standard for mycobiome analysis of clinical samples

Authors

FARNÍKOVÁ, Simona (203 Czech Republic), Kateřina VYKLICKÁ (203 Czech Republic), Petra BRENEROVÁ (203 Czech Republic) and Petra BOŘILOVÁ LINHARTOVÁ (203 Czech Republic, guarantor, belonging to the institution)

Edition

Setkání biochemiků a molekulárních biologů, 2023

Other information

Language

English

Type of outcome

Konferenční abstrakt

Field of Study

10608 Biochemistry and molecular biology

Country of publisher

Czech Republic

Confidentiality degree

není předmětem státního či obchodního tajemství

RIV identification code

RIV/00216224:14310/23:00133554

Organization unit

Faculty of Science

Keywords in English

Microbiome; mycobiome; internal standard; fungi

Změněno: 24/5/2024 10:02, doc. RNDr. Petra Bořilová Linhartová, Ph.D., MBA

Abstract

V originále

The presence of microbial communities in human clinical samples can be studied by DNA sequencing. Unlike bacterial microbiome (bacteriome), which has become a common topic in the literature, fungal microbiome (mycobiome) is relatively rarely studied. Highthroughput sequencing experiments require a mock community as a positive control. Including such control allows us to evaluate the extent to which the sequencing result is biased away from the correct fungal composition of the samples. However, studies using fungal mock communities are not available, although some studies use mock communities in the form of fruiting bodies or spores collected from sporocarps. This work aims to design a fungal internal standard that can be spiked into samples with human DNA while showing no similarities to fungi that might be present in such samples and to suggest a suitable dilution of that internal standard. The sequence of specific fungus was chosen. In the NCBI database, an ITS2 region, into which our chosen primers fit, was defined; the defined single-stranded sequence was commercially obtained. The synthetized ssDNA internal standard sample was cloned to produce dsDNA and the sequence of this DNA was verified by whole genome sequencing. Classic ITS PCR reactions with 1 µl of the internal standard were performed at several dilutions – 1,000×, 100,000×, 200,000×, 500,000×, 800,000× and 1,000,000× to determine the appropriate concentration of the added internal standard to the clinical samples; the quality and quantity control of PCR products was evaluated using electrophoresis and fluorometry. The sequencing of dsDNA confirms successful cloning. The results from gel electrophoresis show robust bands in dilution 1,000×, 100,000×, 200,000×, and 500,000×. However, the bands of 800,000× and 1,000,000× dilution seem appropriate for spiking the clinical samples for sequencing. Nevertheless, since the cloned DNA degraded over time, for future analyses it is necessary to first verify the concentration of the stock DNA by fluorometric measurement and visualize PCR products on a gel electrophoresis. A synthetic fungal internal standard was created that does not interfere with real clinical samples. The dilution 800,000× and 1,000,000× of the internal standard was chosen as appropriate dilution for spiking clinical samples for sequencing. However, the suitability of the selected internal standard dilution must be confirmed by sequencing analysis. Results from this analysis will be further used in the work with clinical samples.

Links

LM2023069, research and development project

Name: Výzkumná infrastruktura RECETOX

Investor: Ministry of Education, Youth and Sports of the CR, RECETOX research infrastructure

Citovat

FARNÍKOVÁ, Simona, Kateřina VYKLICKÁ, Petra BRENEROVÁ and Petra BOŘILOVÁ LINHARTOVÁ. The design of internal standard for mycobiome analysis of clinical samples. In Setkání biochemiků a molekulárních biologů. 2023.

@proceedings{2374664,
   author = {Farníková, Simona and Vyklická, Kateřina and Brenerová, Petra and Bořilová Linhartová, Petra},
   booktitle = {Setkání biochemiků a molekulárních biologů},
   keywords = {Microbiome; mycobiome; internal standard; fungi},
   language = {eng},
   title = {The design of internal standard for mycobiome analysis of clinical samples},
   year = {2023}
}

TY  - CONF
ID  - 2374664
AU  - Farníková, Simona - Vyklická, Kateřina - Brenerová, Petra - Bořilová Linhartová, Petra
PY  - 2023
TI  - The design of internal standard for mycobiome analysis of clinical samples
KW  - Microbiome
KW  - mycobiome
KW  - internal standard
KW  - fungi
N2  - The presence of microbial communities in human clinical samples can be studied by DNA sequencing. Unlike bacterial microbiome (bacteriome), which has become a common topic in the literature, fungal microbiome (mycobiome) is relatively rarely studied. Highthroughput sequencing experiments require a mock community as a positive control. Including such control allows us to evaluate the extent to which the sequencing result is biased away from the correct fungal composition of the samples. However, studies using fungal mock communities are not available, although some studies use mock communities in the form of fruiting bodies or spores collected from sporocarps. This work aims to design a fungal internal standard that can be spiked into samples with human DNA while showing no similarities to fungi that might be present in such samples and to suggest a suitable dilution of that internal standard. The sequence of specific fungus was chosen. In the NCBI database, an ITS2 region, into which our chosen primers fit, was defined; the defined single-stranded sequence was commercially obtained. The synthetized ssDNA internal standard sample was cloned to produce dsDNA and the sequence of this DNA was verified by whole genome sequencing. Classic ITS PCR reactions with 1 µl of the internal standard were performed at several dilutions – 1,000×, 100,000×, 200,000×, 500,000×, 800,000× and 1,000,000× to determine the appropriate concentration of the added internal standard to the clinical samples; the quality and quantity control of PCR products was evaluated using electrophoresis and fluorometry. The sequencing of dsDNA confirms successful cloning. The results from gel electrophoresis show robust bands in dilution 1,000×, 100,000×, 200,000×, and 500,000×. However, the bands of 800,000× and 1,000,000× dilution seem appropriate for spiking the clinical samples for sequencing. Nevertheless, since the cloned DNA degraded over time, for future analyses it is necessary to first verify the concentration of the stock DNA by fluorometric measurement and visualize PCR products on a gel electrophoresis. A synthetic fungal internal standard was created that does not interfere with real clinical samples. The dilution 800,000× and 1,000,000× of the internal standard was chosen as appropriate dilution for spiking clinical samples for sequencing. However, the suitability of the selected internal standard dilution must be confirmed by sequencing analysis. Results from this analysis will be further used in the work with clinical samples.
ER  -

FARNÍKOVÁ, Simona, Kateřina VYKLICKÁ, Petra BRENEROVÁ and Petra BOŘILOVÁ LINHARTOVÁ. The design of internal standard for mycobiome analysis of clinical samples. In \textit{Setkání biochemiků a molekulárních biologů}. 2023.

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