Publications by authors named "Ying-Xu Shi"

Article Synopsis
  • - The study aimed to assess the effectiveness of multiplex PCR combined with capillary electrophoresis (MPCE) for detecting JAK2V617F and CALR mutations in myeloproliferative neoplasms (MPN).
  • - Researchers designed specific primers for both mutations, tested them in one PCR reaction, and found that MPCE could detect JAK2V617F mutations as low as 0.01 ng of genomic DNA.
  • - The results showed 100% consistency between MPCE and a commercial diagnostic kit, suggesting that MPCE could serve as a reliable new method for molecular diagnosis of MPN in patients.
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The proliferation and differentiation of myoblast cells are regulated by the fibroblast growth factor receptor (FGFR) signaling pathway. Although the regulation of FGFR signaling cascades has been widely investigated, the inhibitory mechanism that particularly function in skeletal muscle myogenesis remains obscure. In this study, we determined that LRTM1, an inhibitory regulator of the FGFR signaling pathway, negatively modulates the activation of ERK and promotes the differentiation of myoblast cells.

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Lysine-specific demethylase 1 (LSD1) is a well characterized transcriptional regulator functioning on the chromatin to remove mono- and di-methyl groups from lysine 4 or lysine 9 of histone 3 (H3K4 or H3K9). LSD1 also has non-transcriptional activities via targeting non-histone substrates that participate in diverse biological processes. In this report, we determined that LSD1 negatively regulates autophagy in skeletal muscle cells by promoting PTEN degradation in a transcription-independent mechanism.

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Objective: To investigate the chemotherapeutic efficency of quercetin sensitized adriamycin.

Method: CCK-8 was used to detect the inhibitory effect of different doses of adriamycin, quercetin and quercetin combined with adriamycin on the proliferation of primary leukemia cells from patients with clinically refractory acute leukemia. Quercetin, adriamycin and their combination were used to treat non-irradiated T-ALL leukemia mice to observe the changes of survival curve and myocardial injury.

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Diabetes is a chronic disease that disrupts the balance between bone formation and bone desorption, which can lead to osteoporosis, increasing the risk of fracture. However, compared with osteoblasts, the biological effects of hyperglycemia on osteoclastogenesis remain to be elucidated. Therefore, we investigated the impact of glucose at different concentrations (5.

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Article Synopsis
  • The study aimed to understand how the spleen affects the status of T-cell acute lymphoblastic leukemia (T-ALL) in mice by monitoring leukemia cell development in various organs post-transplantation.
  • It was found that the spleen underwent significant changes during T-ALL progression, with a notable increase in T-ALL cells, and its weight fluctuated more than other organs like the liver.
  • Splenectomy, the surgical removal of the spleen, delayed the progression of T-ALL, indicating that the spleen plays a supportive role in the disease's advancement and serves as a key environment for leukemia cells.
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Aim: We have reported novel anticancer bioactive peptides (ACBPs) that show tumor-suppressive activities in human gastric cancer, leukemia, nasopharyngeal cancer, and gallbladder cancer. In this study, we investigated the effects of ACBPs on human colorectal cancer and the underlying mechanisms.

Methods: Cell growth and apoptosis of human colorectal tumor cell line HCT116 were measured using cell proliferation assay and flow cytometry, respectively.

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This study was purposed to investigate the expression of ADAR1 isoforms of P110 and P150 during the development of murine leukemia. A Notch1 over-expressing murine T cell acute lymphoblastic leukemia model was used to study the expression of ADAR1. BMMNC were isolated at different stages of disease and CD45.

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This study was aimed to investigate the growth and multiple differentiation potential of human umbilical cord tissue derived mesenchymal stem cells (UC-MSCs) transfected by a retroviral vector with catalase (CAT) gene. The UC-MSCs cultured in vitro were transfected by using pMSCV carrying GFP (pMSCV-GFP) and pMSCV carrying CAT (pMSCV-GFP-CAT) respectively, then the MSC-GFP cell line and MSC-GFP-CAT cell line were obtained by sorting of flow cytometry. The GFP expression was observed by a fluorescent microscopy at 48 hours after CAT gene transfection.

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