Autostainer xl platform

Manufactured by Leica

The Autostainer-XL platform is a laboratory equipment designed for automated immunohistochemistry (IHC) and in situ hybridization (ISH) staining. It provides consistent and reliable results through its automated staining process.

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Autostainer XL (183 citations) Autostainer (38 citations)

2 protocols using autostainer xl platform

Histopathological Analysis of Murine Organs

Cited 1 time

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Organs (liver, spleen, and kidney) were harvested from mice and fixed in neutral buffered formalin (10%) and subsequently embedded in paraffin to generate tissue blocks. These blocks were then sectioned at a thickness of 4 µm and stained using Harris hematoxylin (Leica Surgipath) and alcoholic eosin-Y stain (Leica Surgipath). Staining was executed using the automated Leica autostainer-XL platform. Upon staining, the sections were subsequently analyzed by two pathologists on a brightfield microscope to determine morphology and architectural coherence. These pathological assessments were performed in a blinded manner. Detailed and comprehensive analysis of cellular and -subcellular level changes of organs were performed as previously described (16 (link)).

He T., Cheng C., Qiao Y., Cho H., Young E., Mannan R., Mahapatra S., Miner S.J., Zheng Y., Kim N., Zeng V.Z., Wisniewski J.P., Hou S., Jackson B., Cao X., Su F., Wang R., Chang Y., Kuila B., Mukherjee S., Dukare S., Aithal K.B., D.S. S., Abbineni C., Vaishampayan U., Lyssiotis C.A., Parolia A., Xiao L, & Chinnaiyan A.M. (2024). Development of an orally bioavailable mSWI/SNF ATPase degrader and acquired mechanisms of resistance in prostate cancer. Proceedings of the National Academy of Sciences of the United States of America, 121(15), e2322563121.

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Histological Analysis of Mouse Organs

Cited 1 time

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Organs (liver, spleen, and kidney) were harvested from mice and fixed in neutral buffered formalin (10%) and subsequently embedded in paraffin to generate tissue blocks. These blocks were then sectioned at a thickness of 4 μm and stained using Harris haematoxylin (Leica Surgipath) and alcoholic eosin-Y stain (Leica Surgipath). Staining was executed using the automated Leica autostainer-XL platform. Upon staining, the sections were subsequently analyzed by two pathologists on a brightfield microscope to determine morphology and architectural coherence. These pathological assessments were performed in a blinded manner. Detailed and comprehensive analysis of cellular and -subcellular level changes of organs were performed as previously described (16 (link)).

He T., Cheng C., Qiao Y., Cho H., Young E., Mannan R., Mahapatra S., Miner S.J., Zheng Y., Kim N., Zeng V.Z., Wisniewski J.P., Hou S., Jackson B., Cao X., Su F., Wang R., Chang Y., Kuila B., Mukherjee S., Dukare S., Aithal K.B., D.S. S., Abbineni C., Lyssiotis C.A., Parolia A., Xiao L, & Chinnaiyan A.M. (2024). Development of an orally bioavailable mSWI/SNF ATPase degrader and acquired mechanisms of resistance in prostate cancer. bioRxiv.

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