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Tailed templates were ligated to double stranded adaptors prepared with oligonucleotides from the Illumina Customer Sequence Letter (version August 12, 2014, Illumina 2014; Table S1).
To determine the species associated with root samples removed from soil cores, the rbcL genes from DNA of pooled root samples were sequenced using Illumina MiSeq (Illumina, Inc., San Diego, CA) run with rbcL PCR primers from Kress et al. (2009) and Illumina step-out PCR primers from the Illumina Customer Sequence Letter (2012).
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The proposed algorithm does not require rescanning original databases until the accumulative amount of newly added customer sequences exceeds a safety bound, which depends on database size.
In methodological terms, we propose a local search metaheuristic which explores rich solution neighborhoods composed of exchanges of variable-length customer sequences.
To decrease the outbound delivery cost, a new delivery strategy considering synthetical dispatched orders, orders and customers matching, and customer visiting sequence is proposed.
Fig. 1 Graphical representation of a customer transaction sequence Fig. 2 Workflow (a) and its paths (b).
The Precise assays combine molecular and sample indexing in 96- and 384-sample formats, enabling customers to sequence up to 4,608 samples on one sequencing run without investment in new equipment or extensive training.
The assays combine molecular and sample indexing in 96- and 384-sample formats, enabling customers to sequence up to 4,608 samples on one sequencing run without investing in new equipment or extensive training.
On the microfluidic chip, each detection probe consisted of a chemically modified nucleotide "coding" segment complementary to target microRNA (from miRBase, http://microrna.sanger.ac.uk/sequences/) or other RNA (control or customer defined sequences) and a spacer segment of polyethylene glycol to extend the "coding" segment away from the substrate.
On the μParaflo microfluidic chip, each detection probe consisted of a chemically modified nucleotide coding segment complementary to target microRNA (from miRBase, http://microrna.sanger.ac.uk/sequences/) or other RNA (control or customer defined sequences) and a spacer segment of polyethylene glycol to extend the coding segment away from the substrate.
Inside the microfluidic chip, each detection probe consisted of a chemically modified nucleotide-coding segment complementary to target microRNA (from miRBase) or other RNA (control or customer defined sequences).
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