CRISPR/Cas9-mediated LINC00511 knockout strategies, increased apoptosis of breast cancer cells via suppressing antiapoptotic genes

Azadbakht, Narjes; Doosti, Abbas; Jami, Mohammad‐Saeid

doi:10.1186/s12575-022-00171-1

Cited by 18 publications

(4 citation statements)

References 41 publications

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“…This study is the first to use a unique promoter to produce the recombinant omp25 polypeptide in L. lactis . Low pH‐induced expression when cells were grown on glucose shift from the post‐exponential to stationary phases (Zeng et al., 2022 ; Azadbakht et al., 2022 ). Without the use of costly or hazardous exogenous compounds and the ability to recover the protein quickly in subsequent steps, this induction is beneficial as an alternative and cost‐effective tool for the production of heterologous proteins of therapeutic or technological interest.…”

Section: Discussionmentioning

confidence: 99%

Brucella abortus antigen omp25 vaccines: Development and targeting based on Lactococcus lactis

Gouran,

Doosti,

Jami

2023

Veterinary Medicine & Sci

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Background Most Brucella infections take place on mucosal membranes. Therefore, creating vaccinations delivered through the mucosa may be crucial for managing brucellosis. Consequently, we assessed the efficacy of a recombinant oral antigen delivery system based on Lactococcus lactis for Brucella abortus omp25 antigen. Method Oral vaccinations with L. lactis transformed with pNZ8148 variants encoding for omp25 (pNZ8148:omp25) and free‐pNZ8148 were administered to mice. On day 30, following immunization in animal groups, anti‐omp25‐specific IgG1 antibodies were assessed by the ELISA test. Additionally, nasal and bronchoalveolar lavages containing omp25‐specific secretory IgA (sIgA) were analysed by ELISA. ELISA test and real‐time PCR were also used to analyse cytokine responses up to 28 days following the last boost. In addition, the protective potential of L. lactis pNZ8148:omp25 vaccines was assessed in BALB/c mice by exposing them to the B. abortus strain. Results Based on the initial screening results, the omp25 protein was identified for immunogenicity because it had the maximum solubility and flexibility and antigenic values of 0.75. The produced plasmid was digested using KpnI and XbaI. By electrophoretic isolation of the digestion fragments at 786 bp, the omp25 gene, the successful production of the recombinant plasmid, was confirmed. Antigen expression at the protein level revealed that the target group generated the 25 kDa‐sized omp25 protein, but there was no protein expression in the control group. Fourteen days after priming, there was a considerable amount of omp25‐specific IgG1 in the sera of mice vaccinated with pNZ8148–Usp45–omp25–L. lactis (p < 0.001 in target groups compared to the phosphate‐buffered saline control group). IFN‐γ and TNF‐α levels were more significant in samples from mice that had been given the pNZ8148–Usp45–omp25–L. lactis and IRBA vaccinations, in samples taken on days 14 and 28, respectively (p < 0.001). The pNZ8148–Usp45–omp25–L. lactis and IRBA immunization groups had significantly greater IL‐4 and IL‐10 transcription levels than the other groups. The spleen portions from the pNZ8148–Usp45–omp25–L. lactis and IRIBA vac group had less extensive spleen injuries, alveolar oedema, lymphocyte infiltration and morphological damage due to the inflammatory process. Conclusion Our study offers a novel method for using the food‐grade, non‐pathogenic and noncommercial bacterium L. lactis as a protein cell factory to produce the novel immunogenic fusion candidate romp25. This method offers an appealing new approach to assessing the cost‐effective, safe, sustainable, simple pilot development of pharmaceutical products.

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Section: Discussionmentioning

confidence: 99%

Brucella abortus antigen omp25 vaccines: Development and targeting based on Lactococcus lactis

Gouran,

Doosti,

Jami

2023

Veterinary Medicine & Sci

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“…The input parameters for docking analysis were considered ligands and the PDB coordinate file for each protein. The root-mean-square deviation (RMSD) clustering was set at 4Å, and the complex type was modified to the protein–ligand type [ 48 ].…”

Section: Methodsmentioning

confidence: 99%

Use of immunoinformatics and the simulation approach to identify Helicobacter pylori epitopes to design a multi-epitope subunit vaccine for B- and T-cells

Chaleshtori,

Rastegari,

Nayeri

et al. 2023

BMC Biotechnol

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Background Helicobacter pylori cause a variety of gastric malignancies, gastric ulcers, and cause erosive diseases. The extreme nature of the bacterium and the implantation of this bacterium protects it against designing a potent drug against it. Therefore, employing a precise and effective design for a more safe and stable antigenic vaccine against this pathogen can effectively control its associated infections. This study, aimed at improving the design of multiple subunit vaccines against H. pylori, adopts multiple immunoinformatics approaches in combination with other computational approaches. Results In this regard, 10 HTL, and 11 CTL epitopes were employed based on appropriate adopted MHC binding scores and c-terminal cut-off scores of 4 main selected proteins (APO, LeoA, IceA1, and IceA2). An adjuvant was added to the N end of the vaccine to achieve higher stability. For validation, immunogenicity and sensitization of physicochemical analyses were performed. The vaccine could be antigenic with significantly strong interactions with TOLK-2, 4, 5, and 9 receptors. The designed vaccine was subjected to Gromacs simulation and immune response prediction modelling that confirmed expression and immune-stimulating response efficiency. Besides, the designed vaccine showed better interactions with TLK-9. Conclusions Based on our analyses, although the suggested vaccine could induce a clear response against H. pylori, precise laboratory validation is required to confirm its immunogenicity and safety status.

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“…Different CRISPR knock-out approaches (CRISPR-excision, CRISPR-HDR, CRISPR du-HITI) have been used in order to target LINC00511 lncRNA, a long intergenic non-coding RNA overexpressed in breast cancer cells. LINC00511 knock-out leads to important apoptosis rate increase, with an overexpression of proapoptotic genes such as P57 , P21 , PRKCA , MDM4 , MAP2K6 , FADD and downregulation of the antiapoptotic genes BCL-2 and BIRC5 (survivin) [ 61 ].…”

Section: Crispr and Cancermentioning

confidence: 99%

Ten Years of CRISPRing Cancers In Vitro

Capoferri

Filiberti

Faletti

et al. 2022

Cancers

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Cell lines have always constituted a good investigation tool for cancer research, allowing scientists to understand the basic mechanisms underlying the complex network of phenomena peculiar to the transforming path from a healthy to cancerous cell. The introduction of CRISPR in everyday laboratory activity and its relative affordability greatly expanded the bench lab weaponry in the daily attempt to better understand tumor biology with the final aim to mitigate cancer’s impact in our lives. In this review, we aim to report how this genome editing technique affected in the in vitro modeling of different aspects of tumor biology, its several declinations, and analyze the advantages and drawbacks of each of them.

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CRISPR/Cas9-mediated LINC00511 knockout strategies, increased apoptosis of breast cancer cells via suppressing antiapoptotic genes

Cited by 18 publications

References 41 publications

Brucella abortus antigen omp25 vaccines: Development and targeting based on Lactococcus lactis

Brucella abortus antigen omp25 vaccines: Development and targeting based on Lactococcus lactis

Use of immunoinformatics and the simulation approach to identify Helicobacter pylori epitopes to design a multi-epitope subunit vaccine for B- and T-cells

Ten Years of CRISPRing Cancers In Vitro

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