intramolecular recombination
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2021 ◽  
pp. 105140
Author(s):  
Chunkyu Ko ◽  
Jinpeng Su ◽  
Julia Festag ◽  
Romina Bester ◽  
Anna D. Kosinska ◽  
...  

2021 ◽  
Vol 2 ◽  
Author(s):  
Cláudia P. A. Alves ◽  
Duarte Miguel F. Prazeres ◽  
Gabriel A. Monteiro

Minicircles are non-viral delivery vectors with promising features for biopharmaceutical applications. These vectors are plasmid-derived circular DNA molecules that are obtained in vivo in Escherichia coli by the intramolecular recombination of a parental plasmid, which generates a minicircle containing the eukaryotic therapeutic cassette of interest and a miniplasmid containing the prokaryotic backbone. The production process results thus in a complex mixture, which hinders the isolation of minicircle molecules from other DNA molecules. Several strategies have been proposed over the years to meet the challenge of purifying and obtaining high quality minicircles in compliance with the regulatory guidelines for therapeutic use. In minicircle purification, the characteristics of the strain and parental plasmid used have a high impact and strongly affect the purification strategy that can be applied. This review summarizes the different methods developed so far, focusing not only on the purification method itself but also on its dependence on the upstream production strategy used.


2020 ◽  
Vol 22 (2) ◽  
pp. 714-725 ◽  
Author(s):  
Ester Serrano ◽  
Cristina Ramos ◽  
Silvia Ayora ◽  
Juan C. Alonso

2019 ◽  
Vol 12 (1) ◽  
pp. 3586-3598 ◽  
Author(s):  
Alexis R Sullivan ◽  
Yrin Eldfjell ◽  
Bastian Schiffthaler ◽  
Nicolas Delhomme ◽  
Torben Asp ◽  
...  

Abstract Plant mitogenomes can be difficult to assemble because they are structurally dynamic and prone to intergenomic DNA transfers, leading to the unusual situation where an organelle genome is far outnumbered by its nuclear counterparts. As a result, comparative mitogenome studies are in their infancy and some key aspects of genome evolution are still known mainly from pregenomic, qualitative methods. To help address these limitations, we combined machine learning and in silico enrichment of mitochondrial-like long reads to assemble the bacterial-sized mitogenome of Norway spruce (Pinaceae: Picea abies). We conducted comparative analyses of repeat abundance, intergenomic transfers, substitution and rearrangement rates, and estimated repeat-by-repeat homologous recombination rates. Prompted by our discovery of highly recombinogenic small repeats in P. abies, we assessed the genomic support for the prevailing hypothesis that intramolecular recombination is predominantly driven by repeat length, with larger repeats facilitating DNA exchange more readily. Overall, we found mixed support for this view: Recombination dynamics were heterogeneous across vascular plants and highly active small repeats (ca. 200 bp) were present in about one-third of studied mitogenomes. As in previous studies, we did not observe any robust relationships among commonly studied genome attributes, but we identify variation in recombination rates as a underinvestigated source of plant mitogenome diversity.


2019 ◽  
Author(s):  
Alexis R. Sullivan ◽  
Yrin Eldfjell ◽  
Bastian Schiffthaler ◽  
Nicolas Delhomme ◽  
Torben Asp ◽  
...  

AbstractPlant mitogenomes can be difficult to assemble because they are structurally dynamic and prone to intergenomic DNA transfers, leading to the unusual situation where an organelle genome is far outnumbered by its nuclear counterparts. As a result, comparative mitogenome studies are in their infancy and some key aspects of genome evolution are still known mainly from pre-genome, qualitative methods. To help address these limitations, we combined machine learning and in silico enrichment of mitochondrial-like long reads to assemble the bacterial-sized mitogenome of Norway spruce (Pinaceae: Picea abies). We conducted comparative analyses of repeat abundance, intergenomic transfers, substitution and rearrangement rates, and estimated repeat-by-repeat homologous recombination rates. Prompted by our discovery of highly recombinogenic small repeats in P. abies, we assessed the genomic support for the prevailing hypothesis that intramolecular recombination is predominantly driven by repeat length, with larger repeats facilitating DNA exchange more readily. Overall, we found mixed support for this view: recombination dynamics were heterogeneous across vascular plants and highly active small repeats (ca. 200 bp) were present in about a third of studied mitogenomes. As in previous studies, we did not observe any robust relationships among commonly-studied genome attributes, but we identify variation in recombination rates as a underinvestigated source of plant mitogenome diversity.


2018 ◽  
Vol 24 (14) ◽  
pp. 3608-3612 ◽  
Author(s):  
Shao-Chi Lee ◽  
Hsuan-Hung Liao ◽  
Adisak Chatupheeraphat ◽  
Magnus Rueping

2017 ◽  
Vol 23 (49) ◽  
pp. 11771-11775 ◽  
Author(s):  
Xiangqian Liu ◽  
Huifeng Yue ◽  
Jiaqi Jia ◽  
Lin Guo ◽  
Magnus Rueping

2017 ◽  
Vol 19 (16) ◽  
pp. 4255-4258 ◽  
Author(s):  
Adisak Chatupheeraphat ◽  
Hsuan-Hung Liao ◽  
Shao-Chi Lee ◽  
Magnus Rueping

2013 ◽  
Vol 42 (5) ◽  
pp. e37-e37 ◽  
Author(s):  
Hailong Wang ◽  
Xiaoying Bian ◽  
Liqiu Xia ◽  
Xuezhi Ding ◽  
Rolf Müller ◽  
...  

Abstract Recombineering, which is the use of homologous recombination for DNA engineering in Escherichia coli, usually uses antibiotic selection to identify the intended recombinant. When combined in a second step with counterselection using a small molecule toxin, seamless products can be obtained. Here, we report the advantages of a genetic strategy using CcdB as the counterselectable agent. Expression of CcdB is toxic to E. coli in the absence of the CcdA antidote so counterselection is initiated by the removal of CcdA expression. CcdB counterselection is robust and does not require titrations or experiment-to-experiment optimization. Because counterselection strategies necessarily differ according to the copy number of the target, we describe two variations. For multi-copy targets, we use two E. coli hosts so that counterselection is exerted by the transformation step that is needed to separate the recombined and unrecombined plasmids. For single copy targets, we put the ccdA gene onto the temperature-sensitive pSC101 Red expression plasmid so that counterselection is exerted by the standard temperature shift to remove the expression plasmid. To reduce unwanted intramolecular recombination, we also combined CcdB counterselection with Redα omission. These options improve the use of counterselection in recombineering with BACs, plasmids and the E. coli chromosome.


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