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I would suggest you to go with
It is already implied by
Please refer to SPAdes manual: https://cab.spbu.ru/files/release3.15.5/manual.html#sec3.2 both ways are possible. |
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Before using -- isolate, do I need to use --only-error-correction or other NGS reads error correction tools? |
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Well, if this is disabled in |
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I am not exactly convinced that the "--isolate" settings are really the best options to use, even for assumed isolates. Because without an error correction, i am assuming a coverage cutoff is employed to minimize the effect of sequencing errors? Wouldn't that cause the --isolate mode to overlook possible low abundant residual contaminants in assumed "isolates"? |
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I want to assemble the yeast genome, about 11MB-12.5MB. I used PE150 method for sequencing, with high coverage, the coverage >100X. After removing the adapters and filtering low quality base, each read is less than 150bp. The manual indicated that "--isolate flag is highly recommended for high-coverage isolate." At the same time,the article "BENCHMARKING TOOLS FOR DE NOVO MICROBIAL ASSEMBLY" indicated --careful. I noticed that "--isolate option is not compatible with --only-error-correction or --careful options." Only one of these two options can be selected. What should I choose?
In addition, after filtering pair reads (only one library), an unpaired reads file is generated. How should I set input?
-1 <file_name> -2 <file_name> -s <file_name>or
--pe1-1 <file_name> --pe1-2 <file_name> --pe1-s <file_name>After reading the article "BENCHMARKING TOOLS FOR DE NOVO MICROBIAL ASSEMBLY", I got confused. Should I add an option --only-assembler?
Thanks.
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