The MLPA assay and application to diagnosis of DGS The MLPA assay and application to diagnosis of DGS (A) Short regions of DNA, roughly 50–70 bp, are selected as targets, indicated by S and T (1). Single-stranded oligonucleotide probe pairs are designed for each target (2), with half of the target sequence present in the ‘left’ probe and the other half in the ‘right’ probe. Each left probe contains an additional sequence ‘F’ and each right probe contains an additional sequence ‘R’. The right probes also contain a ‘stuffer’ sequence which is a different length for each target to be detected. Genomic DNA is denatured and probes allowed to anneal (3). Annealed probe pairs will lie precisely adjacent to each other on the target DNA (4) allowing DNA ligase to join left and right probes together into a single molecule (5). The ligated probes are denatured away from the target (6), and then PCR amplification is carried out (7) using the same primer pair for all ligated probes (fluorescently-labelled F and the complement of R). The final quantity of each amplified product is dependent upon the copy number of that target sequence within the sample genome. (B) For each target the amount of fluorescent product from the test sample is compared with the amount of product from a control genome, and the ratio is plotted. This plot depicts typical MLPA results for 29 target sequences across the 22q11 region for a patient suspected of having DGS. The gene targeted by each probe is indicated below the plot; distance along the X-axis indicates distance along the chromosome. A ratio of approximately 1.0 indicates normal copy number (blue squares). However the results for 14 targets (including two for the TBX1 gene) give a ratio of only 0.5, indicating a halving of the copy number (one copy instead of the two expected from two complete copies of chromosome 22). This result confirms a diagnosis of DGS. (C) The region of chromosome 22 which is targeted by MLPA probes from the ‘P250-B2 DiGeorge’ kit from MRC-Holland. Cat eye syndrome (CES) is caused by duplication of the region indicated by the green bar; duplications can be identified by amplification ratios of 1.5 compared with control. Roughly 90% of DGS cases result from a 3-Mb deletion, indicated by the blue bar, and including approximately 60 genes, while approximately 8% of cases have a 1.5-Mb deletion, indicated by the purple bar, involving 28 genes. A small number of cases have atypical deletions which may be larger than 3 Mb. While FISH using the TBX1 probe (red) can identify a deletion in the region, MLPA can provide a more accurate picture of the extent of any imbalance due to the greater number of probes used. The P250-B2 DiGeorge kit also contains probes that target relevant regions on chromosomes 4q, 8p, 9q, 10p and 17p, in which copy imbalance generates phenotypes which overlap with DGS; thus a single MLPA assay can assess multiple target regions. Chromosome ideogram from NCBI Genome Decoration Page. Maria Jackson et al. Essays Biochem. 2018;62:643-723 ©2018 by Portland Press Ltd