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Hierarchical DNA Memory based on Nested PCR Satoshi Kashiwamura, Masahito Yamamoto, Atsushi Kameda, Toshikazu Shiba, Azuma Ohuchi.

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Presentation on theme: "Hierarchical DNA Memory based on Nested PCR Satoshi Kashiwamura, Masahito Yamamoto, Atsushi Kameda, Toshikazu Shiba, Azuma Ohuchi."— Presentation transcript:

1 Hierarchical DNA Memory based on Nested PCR Satoshi Kashiwamura, Masahito Yamamoto, Atsushi Kameda, Toshikazu Shiba, Azuma Ohuchi

2 Introduction  Nested Primer Molecular Memory  Data structure of NPMM  Addressing of the data  Merits of NPMM  NPMM design  strategy of primer design  Experiments  dissussion

3 Nested PCR

4 Data structure of NPMM 3 Address block : Ai / Bj / Ck I,j,k ∈ { 0,1,2 } Re : reverse primer (common primer) Example data 101 = A1, B0, C1

5 Addressing of the data 1.Select a p ∈ P and then perform PCR to NPMM with p and Re 2.Select another p’ ∈ P, then perform PCR to the diluted solution after previous PCR. 3.Repeat process 2 for an appropriate number of times

6 Merits of NPMM The level of data security : it is impossible to read data without primers each primer works as a keys each key is independent of other keys A large capacity with a high reaction specificity : M (bit) = 2 * Data(bp) * Primer block M : the memory capacity of NPMM Data : the length of the sequence in the data block Block : the number of address blocks Primer : the number of primers in each address block

7 NPMM design  Size of NPMM : data sequence : 20bp data sequence : 20bp primers : all 15bp primers : all 15bp template : 80bp ( 15 + 15 + 15 + 20 + 15 ) template : 80bp ( 15 + 15 + 15 + 20 + 15 )  Several regards GC content GC content hamming distance hamming distance 3’ end complementary 3’ end complementary  Fitness = GC weight * GC value + H weight * H value + H weight * H value + E weight * E value E weight * E value

8

9 Experiments expected result data 000 = [ Bo, Co ] data 001 = [ Bo, C1 ] data 010 = [ B1, Co ] data 011 = [ B1, C1 ]

10 Amplify the target sequence using Bo or B1 / Re perform 23 cycle denature 94C for 10sec anneal 50C for 30 sec extension 72C for 5 sec using Co or C1 / Re same condition

11 Result 1  Run 10% poly acrylamide gel

12 Detection of amplified sequence 50bp is too short to sequencing ---- need another PCR for detection BoCoData oooRe 5’ end 15 mer

13 Result 2 using data 000 / data 001 data 010 / data 011 primers perform 25 cycle using same condition 10% Poly acrylamide gel

14 Amplify using concatenation primer whether we can extract the target data by once PCR. Anneal 50 C or 58 C or 74 C for 30 sec PCR to NPMM using B0 C0 Detection of the sequence amplified with B0 C0 BoCoData oooRe 1st 2nd 1 st / 2nd

15 Result 3 using data 000 / data 001 data 010 / data 011 primers 10% Poly acrylamide gel

16 Discussion Proposed a DNA memory with A high capacuity / high data security / high specificity.. Future work Scaling up of NPMM Design strategy for set of primers without dependence on the data sequence

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