PrimeFlow RNA assay verified that the sLCL 381 cells are EBV-infected B cells.

PrimeFlow RNA assay verified that the sLCL 381 cells are EBV-infected B cells.

<p>1.5 x 10<sup>6</sup> <b>(a)</b> sLCL 381 and <b>(b)</b> sLCL 421 cells were stained by Aqua Blue dye (Invitrogen, USA) and the following fluorochrome-conjugated antibodies: Pacific Blue anti-human CD3, PE-Cy7 anti-human CD8, PE anti-human CD19, FITC anti-...

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Bibliographic Details
Main Author: Kam Pui Tam (19746865) (author)
Other Authors: Jia Xie (247149) (author), Rex Kwok Him Au-Yeung (19746868) (author), Alan K. S. Chiang (8677455) (author)
Published: 2024
Subjects:
Biochemistry
Medicine
Microbiology
Cell Biology
Molecular Biology
Pharmacology
Immunology
Cancer
Mental Health
Hematology
Infectious Diseases
Virology
transplant lymphoproliferative disorder
latent membrane protein
distinct latency patterns
cause synergistic killing
b signaling pathway
associated hemophagocytic lymphohistiocytosis
nf -&# 954
b &# 945
bortezomib potently induced
xlink "> epstein
latent viral proteins
ebv nuclear antigen
cell cycle arrest
bortezomib prevented lmp
2 causing g1
venetoclax inhibited bcl
viral proteins
&# 954
inhibited mcl
venetoclax targets
venetoclax decreased
taken together
scid mice
proteasome system
proteasome inhibitor
phosphorylated p65
host cells
either lmp
dependent manner
data corroborated
cyclin d1
apoptotic initiator
2 upregulated
2 simultaneously
2 inhibitor
2 family
001 ).
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Summary:<p>1.5 x 10<sup>6</sup> <b>(a)</b> sLCL 381 and <b>(b)</b> sLCL 421 cells were stained by Aqua Blue dye (Invitrogen, USA) and the following fluorochrome-conjugated antibodies: Pacific Blue anti-human CD3, PE-Cy7 anti-human CD8, PE anti-human CD19, FITC anti-human CD16/56 (BioLegend, USA) and PE-Texas Red anti-CD4 (eBioscience, USA) on ice for 30 minutes for indication of cell viability and immunophenotype. The cells were fixed by fixation buffer and subsequently treated with PrimeFlow RNA permeabilization buffer with RNase inhibitors. The EBER in the cells were stained by fluorochrome-conjugated probe EBER-AF647 (Thermo Fisher Scientific, USA) and the cells were incubated in the dark at 4°C overnight. On the next day, the cells were incubated with PrimeFlow RNA PreAmp Mix, PrimeFlow RNA Amp Mix, and diluted Label Probes for signal amplification. The samples were measured by flow cytometry and analyzed by FlowJo software (Tree Star).</p> <p>(TIF)</p>

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