Nanodrop Ratios Explained | 260/280 ratio DNA | 260/280 ratio RNA | 260/230 Ratio | Qunatification |

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  • เผยแพร่เมื่อ 3 ธ.ค. 2022
  • Nanodrop Ratios Explained | 260/280 ratio DNA | 260/280 ratio RNA | 260/230 Ratio | Quantification |
    This video lecture explains
    1. The principle of Nanodrop instrumentation
    2. Ideal 260/280 ratio for DNA and RNA concentration Measurements
    3. Ideal 260/230 ratio for DNA and RNA concentration measurement
    4. Absorption maxima for DNA, RNA, Proteins, and Salts
    5. Real-world examples of RNA and RNA quantification using Nanodrop Instrumentation
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    This video is for educational purposes only. Copyright Disclaimer Under Section 107 of the Copyright Act 1976, allowance is made for "fair use" for purposes such as criticism, comment, news reporting, teaching, scholarship, and research. Fair use is a use permitted by copyright statute that might otherwise be infringing. Non-profit, educational, or personal use tips the balance in favor of fair use.
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ความคิดเห็น • 25

  • @easybiologynotes
    @easybiologynotes ปีที่แล้ว +6

    Very well explained about the basics of ratios for RNA and DNA quantification

  • @investincrypto2859
    @investincrypto2859 ปีที่แล้ว +3

    Very good explanation about nanodrop ratios for DNA RNA quantification

  • @reyhaneesmaieli1117
    @reyhaneesmaieli1117 หลายเดือนก่อน +2

    you explained it so well. thank you

  • @turtle-jelly
    @turtle-jelly ปีที่แล้ว +3

    I understand this perfectly! Thank you!

  • @janhvi143
    @janhvi143 7 หลายเดือนก่อน +1

    very detailed & just what I needed! thank you

  • @dikshyapanthi7681
    @dikshyapanthi7681 ปีที่แล้ว +1

    Excellent lecture you n TH-cam about nanodrop ratios

  • @mohamadhasanansarizadeh7420
    @mohamadhasanansarizadeh7420 7 หลายเดือนก่อน +1

    Thanks, simple and informative, AND CLEAR

    • @BiologyLectures
      @BiologyLectures  7 หลายเดือนก่อน

      Thanks a lot. Your comment means a lot to us. It is highly motivating for us.

  • @michellesuelo7581
    @michellesuelo7581 หลายเดือนก่อน

    hello! may I ask what software you used to graph that?

  • @vkings4life
    @vkings4life ปีที่แล้ว +1

    Thanks alot for this

  • @markrobinson9676
    @markrobinson9676 ปีที่แล้ว +1

    Excellent explanation sir 😊

  • @MohdFaisal-ps7df
    @MohdFaisal-ps7df ปีที่แล้ว +1

    If we have contamination in our extracted DNA or RNA and we don't have extra sample for the extraction again, what should we do in this case how we can decontaminate our extracted DNA?

    • @BiologyLectures
      @BiologyLectures  ปีที่แล้ว

      Enzymes such as DNase or RNase can be used to degrade contaminating DNA or RNA, respectively. If the contaminant is the opposite nucleic acid type (e.g., DNA contaminating an RNA sample), using the appropriate enzyme can help degrade the contaminant while leaving the target nucleic acid relatively intact.

    • @MohdFaisal-ps7df
      @MohdFaisal-ps7df ปีที่แล้ว

      @@BiologyLectures Thanks for the response, i know this but my question is how we will perform this on already extracted DNA or RNA is there any method to perform this, I hope you you don't mind
      Thank you

    • @BiologyLectures
      @BiologyLectures  ปีที่แล้ว

      @@MohdFaisal-ps7df You can perform DNAse or RNAse treatment on already extracted DNA or RNA. Just take already started DNA or RNA and use DNAse or RNAse and corresponding buffer. I hope this helps.

  • @akankshyapattanayak9469
    @akankshyapattanayak9469 8 หลายเดือนก่อน

    Thank You Sir for explaining .
    Sir, If question raises,,, What is 260/280 ratio
    ...... Can we answer that 260 is for DNA and 280 for protein..
    Please reply