Evaluation of Microfluidics-FISH method in prenatal diagnosis

Pietrzyk, Aleksandra; Ryłów, Małgorzata; Bryśkiewicz, Marta; Studniak, Ewa; Piotrowski, Krzysztof; Zajączek, Stanisław; Gronwald, Jacek

doi:10.5603/gp.a2017.0119

Cited by 4 publications

(5 citation statements)

References 9 publications

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“…We used FISH as a representative method to study the feasibility of establishing Levey-Jennings chart-based IQCs for monitoring molecular diagnostic quality, because FISH is widely used to detect aneuploidies after amniocentesis and to perform chromosome analysis of leukemic blood samples and other tissues [20][21][22][23][24]. In general, each clinical sample only includes one karyotype.…”

Section: Discussionmentioning

confidence: 99%

“…Thus, considering that the accuracy of aneuploidy detection by FISH can be improved by increasing cell counts [20][21][22]27], and that quality-control cells containing different proportions of karyotypes can more accurately assess detection quality [26], we used 60 and 20% as the thresholds for aneuploidy detection [28,29]. We prepared high-, medium-, and low-value qualitycontrol cells (A-H) with aneuploidy ratios of 10, 30, 70, and 90%, respectively, to provide a relatively consistent ratio of chimeras to the common clinical samples with various karyotypes as the basis to establish an ideal IQC for prenatal molecular diagnosis by FISH [20][21][22][23][24]. Although the quality-control cells transfected with SV40LT are not identical to primary amniocytes and Phaseolus vulgaris-leucoagglutinin (PHA)-stimulated lymphocytes used for FISH quality control approaches in 26 laboratories [30], they have several advantages as IQCs.…”

Section: Discussionmentioning

confidence: 99%

“…Compared with non-chimeric karyotypes, chimeric karyotypes are more common and are more easily misdiagnosed in prenatal diagnosis by FISH, particularly in individuals with a low proportion of multiple karyotypes [ 24 – 26 ]. Thus, considering that the accuracy of aneuploidy detection by FISH can be improved by increasing cell counts [ 20 – 22 , 27 ], and that quality-control cells containing different proportions of karyotypes can more accurately assess detection quality [ 26 ], we used 60 and 20% as the thresholds for aneuploidy detection [ 28 , 29 ]. We prepared high-, medium-, and low-value quality-control cells (A-H) with aneuploidy ratios of 10, 30, 70, and 90%, respectively, to provide a relatively consistent ratio of chimeras to the common clinical samples with various karyotypes as the basis to establish an ideal IQC for prenatal molecular diagnosis by FISH [ 20 – 24 ].…”

Section: Discussionmentioning

confidence: 99%

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A novel use for Levey-Jennings charts in prenatal molecular diagnosis

Weng

Ying

et al. 2020

BMC Med Genomics

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Background: The goal of this study was to determine whether Levey-Jennings charts, which are widely used in clinical laboratories, can be used to create standardized internal quality controls (IQCs) for prenatal molecular diagnosis. Methods: Aneuploid amniocyte lines with trisomy 13, 21, and 18, and 47,XXY were established by transfection with SV40LTag-pcDNA3.1(−)and combined at different ratios to generate aneuploidy chimeric quality-control cell mixtures A to H. These quality-control cells were then used to calculate the X, X ±1 standard deviation (SD), X ±2 SD, and X ±3 SD values to develop standardized IQCs for methods used for the prenatal diagnosis of aneuploidies such as FISH. Results: Methods for constructing aneuploid amniocyte lines were developed and a set of quality-control cells (A-H) were prepared. The X ±1 SD, X ±2 SD, and X ±3 SD values of these quality-control cells for trisomy 13 and 21

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Section: Discussionmentioning

confidence: 99%

Section: Discussionmentioning

confidence: 99%

Section: Discussionmentioning

confidence: 99%

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A novel use for Levey-Jennings charts in prenatal molecular diagnosis

Weng

Ying

et al. 2020

BMC Med Genomics

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“…Chromosomal preparations were developed according to the method of direct analysis from the chorion and placenta cones of the fetus, which were taken by the majority, after the umbilical cord blood lifocytes and amniocytes were grown in a nutrient medium under a thermostat for 72 hours, and the preparations were also colored according to GTG, CBG methods [12][13][14][15]. The study depends on the time of cultivation after obtaining the working material, the duration of preparation, and analysis.…”

Section: Methodsmentioning

confidence: 99%

Genomic and structural abnormalities of the chromosome set of the fetus, depending on the age of pregnant women

Kalimagambetov

Kalieva

Satybaldieva

et al. 2021

ijbch

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To study the frequency and spectrum of fetal chromosomal abnormalities in pregnant women, depending on age, a cytogenetic study of 2248 biopsies of the chorion and placenta, cord blood lymphocytes and amniocytes was carried out in 2016-2020. The work used the generally accepted methods of direct preparation of chromosome preparation and methods of cell cultivation. The analysis of the preparations was performed based on GTG, CBG staining method and FISH method, using DNA probes for centromeric regions 13, 18, 21 and X, Y chromosomes. Numerical and structural abnormalities of chromosomes were considered according to the ISCN 2013 system. As a result of the study, 272 (12.1%) cases of genomic and structural abnormalities of the fetus chromosomes of the fetus of pregnant women were registered. Genomic abnormalities were 69.1%, and chromosome structural rearrangements -30.9%. Among genomic disorders, the frequency of the Down syndrome in the karyotype of the fetus was 58.5%. Frequency of occurrence of fetal chromosomal abnormalities varies significantly depending on the age group of pregnant women. The frequency of fetal chromosomal pathology in pregnant women under 20 years old was 4.4%, at the age from 20 to 34 years old -7.6%, from 35 to 39 years old -16.3%, from 40 to 44 years old -19.8%, after 45 years figure increased significantly -up to 29.6%. In older pregnant women, when compared with pregnant women of the reproductive period from 20 to 34 years, when the highest level of pregnancy rate (54.6%) in the population is observed, there is an increase in the frequency of fetal chromosomal pathology by 2.1; 2.6 and 3.9 times, respectively.

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“…These techniques provided additional information with which to predict the overall genetic condition of the developing fetus [ [7] , [8] , [9] , [10] ]. Karyotyping and FISH have become the low-cost gold standard in prenatal screening of numerous chromosomal anomalies [ 11 , 12 ]. However, karyotyping and FISH exhibit certain limitations such as the need of a skilled analysts like cytogeneticists or clinical specialists who can obtain a tissue sample safely without harming the fetus.…”

Section: Expanding Scope Of Non-invasive Prenatal Screeningmentioning

confidence: 99%