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متن کامل


نویسندگان: 

LIU D. | REN T. | GAO X.

اطلاعات دوره: 
  • سال: 

    2003
  • دوره: 

    10
  • شماره: 

    14
  • صفحات: 

    1307-1315
تعامل: 
  • استنادات: 

    1
  • بازدید: 

    161
  • دانلود: 

    0
کلیدواژه: 
چکیده: 

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بازدید 161

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نویسندگان: 

نشریه: 

Curr Protoc Chem Biol

اطلاعات دوره: 
  • سال: 

    2017
  • دوره: 

    9
  • شماره: 

    3
  • صفحات: 

    147-157
تعامل: 
  • استنادات: 

    1
  • بازدید: 

    175
  • دانلود: 

    0
کلیدواژه: 
چکیده: 

شاخص‌های تعامل:   مرکز اطلاعات علمی Scientific Information Database (SID) - Trusted Source for Research and Academic Resources

بازدید 175

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اطلاعات دوره: 
  • سال: 

    2020
  • دوره: 

    15
  • شماره: 

    5
  • صفحات: 

    437-446
تعامل: 
  • استنادات: 

    0
  • بازدید: 

    97
  • دانلود: 

    0
چکیده: 

Background and purpose: The optimization of an effective non-viral gene delivery method for genetic manipulation of primary human T cells has been a major challenge in immunotherapy researches. Due to the poor Transfection efficiency of conventional methods in T cells, there has been an effort to increase the Transfection rate in these cells. Protamine is an FDA-approved compound with a documented safety profile that enhances DNA condensation for gene delivery. Experimental approach: In this study, the effect of protamine sulfate on the Transfection efficiency of standard Transfection reagents, was evaluated to transfect primary human T cells. In this regard, pre-condensation of DNA was applied using protamine, and the value of the zeta potential of DNA/protamine/cargo complexes was determined. T cells were transfected with DNA/protamine/cargo complexes. The Transfection efficiency rate was evaluated by flow cytometry. Also, the green fluorescent protein expression level and cytotoxicity of each complex were identified using real-time polymerase chain reaction and MTT assay, respectively. Findings/Results: Our results demonstrated that protamine efficiently increases the positive charge of DNA/cargo complex without any cytotoxic effect on the primary human T cells. We observed that the Transfection efficiency in DNA/protamine/ Lipofectamine ® 2000 and DNA/protamine/TurboFect TM was 87. 2% and 78. 9%, respectively, while Transfection of T cells by Lipofectamine ® 2000 and TurboFect TM would not result in sufficient Transfection. Conclusion and implications: Protamine sulfate enhanced the Transfection rate of T cells; and could be a promising non-viral gene delivery method to achieve a safe, rapid, cost-effective, and efficient system which will be further applied in gene therapy and T cells manipulation methods.

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مرکز اطلاعات علمی Scientific Information Database (SID) - Trusted Source for Research and Academic Resources
اطلاعات دوره: 
  • سال: 

    2010
  • دوره: 

    2
  • شماره: 

    3
  • صفحات: 

    123-130
تعامل: 
  • استنادات: 

    0
  • بازدید: 

    366
  • دانلود: 

    0
چکیده: 

Purification and isolation of cellular target proteins for monoclonal antibody (MAb) production is a difficult and time-consuming process. Immunization of mice with murine cell lines stably transfected with genes coding for xenogenic target molecules is an alternative method for mouse immunization and MAb production. Here we present data on Transfection efficiency of some commercial reagents used for Transfection of murine myeloma cell lines. Little is known about transfectability of murine myeloma cell lines by different Transfection reagents. Mouse myeloma cell lines (SP2/0, NS0, NS1, Ag8, and P3U1) were transfected with pEGFP-N1 vector using Lipofectamine 2000, jetPEI and LyoVec commercial Transfection reagents in different combinations. The Transfection permissible HEK293-FT cell line was used as a control in Transfection procedure. Transfected cells, expressing the Enhanced Green Fluorescent Protein (EGFP), were analyzed by flow cytometry 48 hrs post Transfection. Our results showed Transfection efficiency of 71%, 57% and 22% for HEK293-FT, 5.5%, 3.4% and 1% for SP2/0, 55.7%, 21.1% and 9.3% for NS0, 8.2%, 6% and 5.5% for NS1, 22%, 49.2% and 5.5% for Ag8 and 6.3%, 21.5% and 4.6% for P3U1 cell lines after Transfection with Lipofectamine 2000, jetPEI and LyoVec reagents, respectively. Our data indicate that NS0 and Ag8 are efficiently transfected by Lipofectamine 2000 and jetPEI reagents. Finally, we propose Ag8 and NS0 cell lines as suitable host cells for efficient expression of target genes which can be used for mouse immunization and MAb production.

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اطلاعات دوره: 
  • سال: 

    1392
  • دوره: 

    21
تعامل: 
  • بازدید: 

    246
  • دانلود: 

    86
چکیده: 

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نویسندگان: 

PEISTER A. | MELLAD J.A.

نشریه: 

GENE THERAPY

اطلاعات دوره: 
  • سال: 

    2004
  • دوره: 

    11
  • شماره: 

    2
  • صفحات: 

    224-228
تعامل: 
  • استنادات: 

    1
  • بازدید: 

    125
  • دانلود: 

    0
کلیدواژه: 
چکیده: 

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بازدید 125

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مرکز اطلاعات علمی Scientific Information Database (SID) - Trusted Source for Research and Academic Resources
اطلاعات دوره: 
  • سال: 

    1978
  • دوره: 

    163
  • شماره: 

    2
  • صفحات: 

    181-187
تعامل: 
  • استنادات: 

    1
  • بازدید: 

    176
  • دانلود: 

    0
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بازدید 176

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اطلاعات دوره: 
  • سال: 

    2004
  • دوره: 

    245
  • شماره: 

    -
  • صفحات: 

    67-82
تعامل: 
  • استنادات: 

    1
  • بازدید: 

    171
  • دانلود: 

    0
کلیدواژه: 
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نشریه: 

Cell Journal (Yakhteh)

اطلاعات دوره: 
  • سال: 

    2008
  • دوره: 

    10
  • شماره: 

    SUPPLEMENT 1
  • صفحات: 

    48-48
تعامل: 
  • استنادات: 

    0
  • بازدید: 

    284
  • دانلود: 

    0
چکیده: 

Objective: (i) if using chemical reagents such as DMSO and Lipofectamine™2000 increase bovine sperm Transfection, (ii) if motile spermatozoa have a greater Transfection rate than immotile ones, and (iii) if increasing sperm- DNA incubation time enhance sperm Transfection rate.Materials and Methods: Motile bull sperms were allowed to swim up at 38oC for 90 min. The rhodamine labeled pGeneGrip-Lac-Z vector (Genelantic, USA) was used for direct detection of transfected cells under epiflourescence microscope. One and three microlitersof Lipofectamine2000 were added separately into two tubes containing 20μl of SP-TALP medium (BSA and antibiotic free) and stored at room temperature for 30 min. One microgram of the vector was added to liposomes and stored at room temperature for a further 90 min to perform 1:1 and 1:3 (DNA: Lipofectamine) ratios. one mg of naked DNA was added into SP-TALP medium as control group and supplemented with 1% and 3% Dimethyl sulfoxide(DMSO) as DMSO groups. for all groups, 1×106 fully capacitated spermatozoa was added to each tube and the total volume adjusted to 30ml with SP-TALP medium (containing 6% BSA) and incubated at 38oC for 60 min. Sperm-DNA mixtures were divided into two groups, treated with or without DNaseI (5 UI) for 30 min and used for fluorescence detection. In another

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نشریه: 

STEM CELLS

اطلاعات دوره: 
  • سال: 

    2004
  • دوره: 

    22
  • شماره: 

    4
  • صفحات: 

    531-543
تعامل: 
  • استنادات: 

    1
  • بازدید: 

    115
  • دانلود: 

    0
کلیدواژه: 
چکیده: 

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بازدید 115

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