Investigating the Pathogenesis of MYH7 Mutation Gly823Glu in Familial Hypertrophic Cardiomyopathy using a Mouse Model

2.9K Views

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03:45 min

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August 8th, 2022

DOI :

10.3791/63949-v

August 8th, 2022

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Yu Xia*¹^,², Jinlin Hu*³, Xiang Li⁴, Shuang Zheng⁴, Ge Wang¹^,², Songtao Tan¹^,², Zengxiao Zou¹^,², Qiong Ling²^,⁵, Fenghua Yang⁴, Xiaoping Fan¹^,²

¹Department of Cardiovascular Surgery, Guangdong Provincial Hospital of Traditional Chinese Medicine, the Second Affiliated Hospital of Guangzhou University of Chinese Medicine, ²The Second Clinical College of Guangzhou University of Chinese Medicine, ³Department of Cardiovascular Surgery, The First Affiliated Hospital, Jinan University, ⁴Guangdong Provincial Key Laboratory of Laboratory Animals, Guangdong Laboratory Animals Monitoring Institute, ⁵Department of Anesthesiology, Guangdong Provincial Hospital of Chinese Medicine, the Second Affiliated Hospital of Guangzhou University of Chinese Medicine

Transcript

This protocol is significant as it can provide a demonstration of ultrasound in small animals. This technique may provide insights into the discovery of pathogenic genes in hereditary cardiomyopathy. Fix the knockin mice horizontally on the platform then tilt the platform 30 degrees coddle to the knockin mouse.

Remove hair on the anterior chest wall of the knockin mice using a depilatory cream position the probe vertically with the bump facing the animal's head. Then rotate the probe counterclockwise approximately 45 degrees in the para sternal long axis view. Rotate the probe 90 degrees clockwise to obtain the para sternal short axis view.

After rotating the probe, adjust the Y axis displacement to get the correct slice. Observe the long axis image of the heart and then select M mode measurement data. Acquire ultrasound data from para sternal long axis views of mice and measure the heart rate, left ventricular ejection fraction, cardiac output, left ventricular and diastolic dimension, left ventricular and systolic dimension.

Left ventricular posterior wall and ventricular septum. The family pedigrees of hypertrophic cardiomyopathy were obtained, and all the documented family members were diagnosed with hypertrophic cardiomyopathy enrollment. Sanger sequencing confirmed the same M Y H 7 P G 8 23 E variant in all patients, but not in the healthy individuals in the families.

And 174 controls, the heterozygous M Y H 7 P G 8 23 E completely co segregated in this family. The glycine residue at Codon 8 23 in the neck domain region of M Y H 7 was highly conserved in all the available vertebrate myocin sequences. According to A C M G standards and guidelines the M Y H 7 P G 8 23 E variant was predicted to be a pathogenic variant.

The knockin mice developed age-dependent cardiac hypertrophy after birth. Echocardiography revealed that the inter ventricular septum and left ventricular posterior wall developed with increased heart rate in the knockin mice. Also confirmed by the histological analysis.

Virus ultrasound data can be obtained by rotating the probe at different angles on different sections of the mouse term.

Summary

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Familial Hypertrophic Cardiomyopathy