Nothing
####### for compare2Sequences
.searchHitsInOneSeq3 <- function(gRNAs, seqs, seqname,
PAM = "NGG", PAM.pattern = "NNN$", PAM.size = 3,
max.mismatch = 2, outfile, allowed.mismatch.PAM = 2,
PAM.location = "3prime", gRNA.size = 20,
baseEditing = FALSE, targetBase = "C", editingWindow = 4:8)
{
if (.preprocess_me2(gRNAs, max.mismatch)) {
patterns <- PDict(gRNAs, max.mismatch = max.mismatch)
} else {
patterns <- gRNAs
}
all_plus_matches <- matchPDict(patterns, seqs,
max.mismatch = max.mismatch)
revseq <- reverseComplement(seqs)
all_minus_matches <- matchPDict(patterns, revseq,
max.mismatch = max.mismatch)
for (i in seq_len(length(gRNAs))) {
patternID <- gsub("'", "", names(gRNAs)[i])
if (length(patternID) < 1) {
patternID <- paste("pattern", i, sep = "")
}
pattern1 <- gRNAs[[i]]
### by default PAM is NGG or NAG
plus_matches <- Views(seqs, all_plus_matches[[i]])
if (length(plus_matches) > 0) {
names(plus_matches) <- rep.int(patternID, length(plus_matches))
writeHits(gRNA = pattern1, seqname = seqname,
matches = plus_matches, strand = "+",
file = outfile, gRNA.size = gRNA.size,
PAM = PAM, PAM.pattern = PAM.pattern,
max.mismatch = max.mismatch,
chrom.len = length(seqs), append = TRUE,
PAM.location = PAM.location,
PAM.size = PAM.size,
allowed.mismatch.PAM = allowed.mismatch.PAM,
seqs = seqs,
baseEditing = baseEditing, targetBase = targetBase, editingWindow = editingWindow)
}
if (reverseComplement(pattern1) != pattern1) {
minus_matches <- Views(revseq, all_minus_matches[[i]])
if (length(minus_matches) > 0) {
names(minus_matches) <- rep.int(patternID,
length(minus_matches))
writeHits(gRNA = pattern1, seqname = seqname,
matches = minus_matches, strand = "-",
file = outfile, gRNA.size = gRNA.size,
PAM = PAM, PAM.pattern = PAM.pattern,
max.mismatch = max.mismatch,
chrom.len = length(seqs), append = TRUE,
PAM.location = PAM.location, PAM.size = PAM.size,
allowed.mismatch.PAM = allowed.mismatch.PAM,
seqs = revseq,
baseEditing = baseEditing, targetBase = targetBase, editingWindow = editingWindow)
}
}
}
}
searchHits <-
function (gRNAs,seqs,seqname,
max.mismatch = 3, PAM.size = 3, gRNA.size = 20,
PAM = "NGG", PAM.pattern = "NNN$",
allowed.mismatch.PAM = 2, PAM.location = "3prime",
outfile,
baseEditing = FALSE, targetBase = "C", editingWindow = 4:8)
{
if (missing(gRNAs) || class(gRNAs) != "DNAStringSet") {
stop("gRNAs is required as a DNAStringSet object!")
}
if (missing(seqs) || class(seqs) != "DNAString") {
stop("seq is required as a DNAString object!")
}
if (width(gRNAs)[1] == (gRNA.size + PAM.size))
{
if(PAM.location == "3prime")
gRNAs <- subseq(gRNAs, 1, gRNA.size)
else
gRNAs <- subseq(gRNAs, PAM.size + 1, gRNA.size + PAM.size)
}
else if (width(gRNAs)[1] != gRNA.size)
{
stop("the gRNA length needs to be equal to the
specified gRNA.size (or gRNA.size plus PAM.size\n)");
}
cat(">>> Finding all hits in sequence", seqname, "...\n")
.searchHitsInOneSeq3(gRNAs = gRNAs, seqs = seqs,
seqname = seqname,
PAM = PAM, gRNA.size = gRNA.size,
PAM.pattern = PAM.pattern, PAM.size = PAM.size,
max.mismatch = max.mismatch, outfile,
allowed.mismatch.PAM = allowed.mismatch.PAM,
PAM.location = PAM.location,
baseEditing = baseEditing, targetBase = targetBase, editingWindow = editingWindow)
cat(">>> DONE searching\n")
if (file.exists(outfile))
{
hits <- read.table(outfile, sep="\t", header = TRUE,
stringsAsFactors = FALSE)
unlink(outfile)
hits
}
else
{
warning("No matching found, please check your input sequence, and make
sure you are using the right genome. You can also alter your
search criteria such as increasing max.mismatch!")
data.frame()
}
}
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