Redirection
Last updated on 2024-05-09 | Edit this page
Estimated time: 45 minutes
Overview
Questions
- How can I search within files?
- How can I combine existing commands to do new things?
Objectives
- Employ the
grep
command to search for information within files. - Print the results of a command to a file.
- Construct command pipelines with two or more stages.
- Use
for
loops to run the same command for several input files.
Searching files
We discussed in a previous episode how to search within a file using
less
. We can also search within files without even opening
them, using grep
. grep
is a command-line
utility for searching plain-text files for lines matching a specific set
of characters (sometimes called a string) or a particular pattern (which
can be specified using something called regular expressions). We’re not
going to work with regular expressions in this lesson, and are instead
going to specify the strings we are searching for. Let’s give it a
try!
Nucleotide abbreviations
The four nucleotides that appear in DNA are abbreviated
A
, C
, T
and G
.
Unknown nucleotides are represented with the letter N
. An
N
appearing in a sequencing file represents a position
where the sequencing machine was not able to confidently determine the
nucleotide in that position. You can think of an N
as being
aNy nucleotide at that position in the DNA sequence.
We’ll search for strings inside of our fastq files. But first, we’re
going to make some symlinks. If you’re a Mac user, you may be familiar
with right-click to Make Alias
; On Windows, you’d
right-click to Create Shortcut
. A symlink points to a file
without making another copy. NOT copying large files saves money on
storage costs!
BASH
$ ln -s /broad/hptmp/computing_basics/untrimmed_fastq/SRR098026.fastq SRR098026.fastq
$ ln -s /broad/hptmp/computing_basics/untrimmed_fastq/SRR097977.fastq SRR097977.fastq
$ ls -F
OUTPUT
SRR097977.fastq@ SRR098026.fastq@ cb_unix_shell/ cb_unix_shell.tgz
Suppose we want to see how many reads in our file have really bad segments containing 10 consecutive unknown nucleotides (Ns).
Determining quality
In this lesson, we’re going to be manually searching for strings of
N
s within our sequence results to illustrate some
principles of file searching. It can be really useful to do this type of
searching to get a feel for the quality of your sequencing results,
however, in your research you will most likely use a bioinformatics tool
that has a built-in program for filtering out low-quality reads. You’ll
learn how to use one such tool in a
later lesson.
Let’s search for the string NNNNNNNNNN in the SRR098026 file:
This command returns a lot of output to the terminal. Every single line in the SRR098026 file that contains at least 10 consecutive Ns is printed to the terminal, regardless of how long or short the file is. We may be interested not only in the actual sequence which contains this string, but in the name (or identifier) of that sequence. We discussed in a previous lesson that the identifier line immediately precedes the nucleotide sequence for each read in a FASTQ file. We may also want to inspect the quality scores associated with each of these reads. To get all of this information, we will return the line immediately before each match and the two lines immediately after each match.
We can use the -B
argument for grep to return a specific
number of lines before each match. The -A
argument returns
a specific number of lines after each matching line. Here we want the
line before and the two lines after each matching
line, so we add -B1 -A2
to our grep command:
One of the sets of lines returned by this command is:
OUTPUT
@SRR098026.599947 HWUSI-EAS1599_1:2:4:1280:2025 length=35
TCANNNNNNNNNNNNNNNNNNNNNNNNNNNNNNNN
+SRR098026.599947 HWUSI-EAS1599_1:2:4:1280:2025 length=35
###!!!!!!!!!!!!!!!!!!!!!!!!!!!!!!!!
Exercise
Search for the sequence
GNATNACCACTTCC
in theSRR098026.fastq
file. Have your search return all matching lines and the name (or identifier) for each sequence that contains a match.Search for the sequence
AAGTT
in both FASTQ files. Have your search return all matching lines and the name (or identifier) for each sequence that contains a match.
grep -B1 GNATNACCACTTCC SRR098026.fastq
@SRR098026.245 HWUSI-EAS1599_1:2:1:2:801 length=35
GNATNACCACTTCCAGTGCTGANNNNNNNGGGATG
grep -B1 AAGTT *.fastq
SRR097977.fastq-@SRR097977.11 209DTAAXX_Lenski2_1_7:8:3:247:351 length=36
SRR097977.fastq:GATTGCTTTAATGAAAAAGTCATATAAGTTGCCATG
--
SRR097977.fastq-@SRR097977.67 209DTAAXX_Lenski2_1_7:8:3:544:566 length=36
SRR097977.fastq:TTGTCCACGCTTTTCTATGTAAAGTTTATTTGCTTT
--
SRR097977.fastq-@SRR097977.68 209DTAAXX_Lenski2_1_7:8:3:724:110 length=36
SRR097977.fastq:TGAAGCCTGCTTTTTTATACTAAGTTTGCATTATAA
[...clip...]
SRR098026.fastq-@SRR098026.599758 HWUSI-EAS1599_1:2:4:1278:392 length=35
SRR098026.fastq:TCAATGCCGGGCAAGTTCGTACAACACGTAGTGCA
--
SRR098026.fastq-@SRR098026.599795 HWUSI-EAS1599_1:2:4:1278:616 length=35
SRR098026.fastq:GTGAGATTGGGAAAGTTTGCACTCATGGGGGAAGG
--
SRR098026.fastq-@SRR098026.599944 HWUSI-EAS1599_1:2:4:1280:742 length=35
SRR098026.fastq:ACAAGAAGTTAACAACCATATAACCTGCACAGGAC
Redirecting output
grep
allowed us to identify sequences in our FASTQ files
that match a particular pattern. All of these sequences were printed to
our terminal screen, but in order to work with these sequences and
perform other operations on them, we will need to capture that output in
some way.
We can do this with something called “redirection”. The idea is that we are taking what would ordinarily be printed to the terminal screen and redirecting it to another location. In our case, we want to print this information to a file so that we can look at it later and use other commands to analyze this data.
The command for redirecting output to a file is
>
.
Let’s try out this command and copy all the records (including all
four lines of each record) in our FASTQ files that contain ‘NNNNNNNNNN’
to another file called bad_reads.txt
.
File extensions
You might be confused about why we’re naming our output file with a
.txt
extension. After all, it will be holding FASTQ
formatted data that we’re extracting from our FASTQ files. Won’t it also
be a FASTQ file? The answer is, yes - it will be a FASTQ file and it
would make sense to name it with a .fastq
extension.
However, using a .fastq
extension will lead us to problems
when we move to using wildcards later in this episode. We’ll point out
where this becomes important. For now, it’s good that you’re thinking
about file extensions!
The prompt should sit there a little bit, and then it should look
like nothing happened. But type ls
. You should see a new
file called bad_reads.txt
.
We can check the number of lines in our new file using a command
called wc
. wc
stands for word
count. This command counts the number of words, lines, and
characters in a file. The FASTQ file may change over time, so given the
potential for updates, make sure your file matches your instructor’s
output.
As of Sept. 2020, wc gives the following output:
OUTPUT
68623 124599 2641459 bad_reads.txt
This will tell us the number of lines, words and characters in the
file. If we want only the number of lines, we can use the
-l
flag for lines
.
OUTPUT
68623 bad_reads.txt
Exercise
How many sequences are there in SRR098026.fastq
?
Remember that every sequence is formed by four lines.
OUTPUT
2400000
Now you can divide this number by four to get the number of sequences in your fastq file.
This can be done using shell integer arithmetic
Note, this will do integer division - if you need floating point arithmetic you can use bc - an arbitrary precision calculator
OUTPUT
600000
Exercise
How many sequences in SRR098026.fastq
contain at least 3
consecutive Ns?
We might want to search multiple FASTQ files for sequences that match
our search pattern. However, we need to be careful, because each time we
use the >
command to redirect output to a file, the new
output will replace the output that was already present in the file.
This is called “overwriting” and, just like you don’t want to overwrite
your video recording of your kid’s first birthday party, you also want
to avoid overwriting your data files.
OUTPUT
68623 bad_reads.txt
OUTPUT
523 bad_reads.txt
Here, the output of our second call to wc
shows that we
no longer have 68623 lines in our bad_reads.txt
file. This
is because the second file we searched (SRR097977.fastq
)
only has 523 lines that match our search sequence. So our file was
overwritten.
We can avoid overwriting our files by using the command
>>
. >>
is known as the “append
redirect” and will append new output to the end of a file, rather than
overwriting it.
OUTPUT
68623 bad_reads.txt
OUTPUT
69146 bad_reads.txt
The output of our second call to wc
shows that we have
added more bad reads to our original data.
We can also do this with a single line of code by using a wildcard:
OUTPUT
69147 bad_reads.txt
Pilot Unix workshop edits stop here
File extensions - part 2
This is where we would have trouble if we were naming our output file
with a .fastq
extension. If we already had a file called
bad_reads.fastq
(from our previous grep
practice) and then ran the command above using a .fastq
extension instead of a .txt
extension, grep
would give us a warning.
OUTPUT
grep: input file ‘bad_reads.fastq' is also the output
grep
is letting you know that the output file
bad_reads.fastq
is also included in your grep
call because it matches the *.fastq
pattern. Be careful
with this as it can lead to some unintended results.
Since we might have multiple different criteria we want to search
for, creating a new output file each time has the potential to clutter
up our workspace. We also thus far haven’t been interested in the actual
contents of those files, only in the number of reads that we’ve found.
We created the files to store the reads and then counted the lines in
the file to see how many reads matched our criteria. There’s a way to do
this, however, that doesn’t require us to create these intermediate
files - the pipe command (|
).
This is probably not a key on your keyboard you use very much, so
let’s all take a minute to find that key. In the UK and US keyboard
layouts, and several others, the |
character can be found
using the key combination Shift+</kbd>. This may
be different for other language-specific layouts.
What |
does is take the output that is scrolling by on
the terminal and uses that output as input to another command. When our
output was scrolling by, we might have wished we could slow it down and
look at it, like we can with less
. Well it turns out that
we can! We can redirect our output from our grep
call
through the less
command.
We can now see the output from our grep
call within the
less
interface. We can use the up and down arrows to scroll
through the output and use q
to exit less
.
If we don’t want to create a file before counting lines of output
from our grep
search, we could directly pipe the output of
the grep search to the command wc -l
. This can be helpful
for investigating your output if you are not sure you would like to save
it to a file.
Because we asked grep
for all four lines of each FASTQ
record, we need to divide the output by four to get the number of
sequences that match our search pattern. Since 802 / 4 = 200.5 and we
are expecting an integer number of records, there is something added or
missing in bad_reads.txt
. If we explore
bad_reads.txt
using less
, we might be able to
notice what is causing the uneven number of lines. Luckily, this issue
happens by the end of the file so we can also spot it with
tail
.
OUTPUT
@SRR098026.133 HWUSI-EAS1599_1:2:1:0:1978 length=35
ANNNNNNNNNTTCAGCGACTNNNNNNNNNNGTNGN
+SRR098026.133 HWUSI-EAS1599_1:2:1:0:1978 length=35
#!!!!!!!!!##########!!!!!!!!!!##!#!
--
--
@SRR098026.177 HWUSI-EAS1599_1:2:1:1:2025 length=35
CNNNNNNNNNNNNNNNNNNNNNNNNNNNNNNNNNN
+SRR098026.177 HWUSI-EAS1599_1:2:1:1:2025 length=35
#!!!!!!!!!!!!!!!!!!!!!!!!!!!!!!!!!!
The fifth and six lines in the output display “–” which is the
default action for grep
to separate groups of lines
matching the pattern, and indicate groups of lines which did not match
the pattern so are not displayed. To fix this issue, we can redirect the
output of grep to a second instance of grep
as follows.
BASH
$ grep -B1 -A2 NNNNNNNNNN SRR098026.fastq | grep -v '^--' > bad_reads.fastq
$ tail bad_reads.fastq
OUTPUT
+SRR098026.132 HWUSI-EAS1599_1:2:1:0:320 length=35
#!!!!!!!!!##########!!!!!!!!!!##!#!
@SRR098026.133 HWUSI-EAS1599_1:2:1:0:1978 length=35
ANNNNNNNNNTTCAGCGACTNNNNNNNNNNGTNGN
+SRR098026.133 HWUSI-EAS1599_1:2:1:0:1978 length=35
#!!!!!!!!!##########!!!!!!!!!!##!#!
@SRR098026.177 HWUSI-EAS1599_1:2:1:1:2025 length=35
CNNNNNNNNNNNNNNNNNNNNNNNNNNNNNNNNNN
+SRR098026.177 HWUSI-EAS1599_1:2:1:1:2025 length=35
#!!!!!!!!!!!!!!!!!!!!!!!!!!!!!!!!!!
The -v
option in the second grep
search
stands for --invert-match
meaning grep
will
now only display the lines which do not match the searched pattern, in
this case '^--'
. The caret (^
) is an
anchoring character matching the beginning of the line,
and the pattern has to be enclose by single quotes so grep
does not interpret the pattern as an extended option (starting with
–).
Custom grep
control
Use man grep
to read more about other options to
customize the output of grep
including extended options,
anchoring characters, and much more.
Redirecting output is often not intuitive, and can take some time to get used to. Once you’re comfortable with redirection, however, you’ll be able to combine any number of commands to do all sorts of exciting things with your data!
None of the command line programs we’ve been learning do anything all that impressive on their own, but when you start chaining them together, you can do some really powerful things very efficiently.
File manipulation and more practices with pipes
To practice a bit more with the tools we’ve added to our tool kit so far and learn a few extra ones you can follow this extra lesson which uses the SRA metadata file.
Writing for loops
Loops are key to productivity improvements through automation as they allow us to execute commands repeatedly. Similar to wildcards and tab completion, using loops also reduces the amount of typing (and typing mistakes). Loops are helpful when performing operations on groups of sequencing files, such as unzipping or trimming multiple files. We will use loops for these purposes in subsequent analyses, but will cover the basics of them for now.
When the shell sees the keyword for
, it knows to repeat
a command (or group of commands) once for each item in a list. Each time
the loop runs (called an iteration), an item in the list is assigned in
sequence to the variable, and the commands inside the
loop are executed, before moving on to the next item in the list. Inside
the loop, we call for the variable’s value by putting $
in
front of it. The $
tells the shell interpreter to treat the
variable as a variable name and substitute its value in
its place, rather than treat it as text or an external command. In shell
programming, this is usually called “expanding” the variable.
Sometimes, we want to expand a variable without any whitespace to its
right. Suppose we have a variable named foo
that contains
the text abc
, and would like to expand foo
to
create the text abcEFG
.
The interpreter is trying to expand a variable named
fooEFG
, which (probably) doesn’t exist. We can avoid this
problem by enclosing the variable name in braces ({
and
}
, also called “curly brackets”). bash
treats
the #
character as a comment character. Any text on a line
after a #
is ignored by bash when evaluating the text as
code.
Let’s write a for loop to show us the first two lines of the fastq
files we downloaded earlier. You will notice the shell prompt changes
from $
to >
and back again as we were
typing in our loop. The second prompt, >
, is different
to remind us that we haven’t finished typing a complete command yet. A
semicolon, ;
, can be used to separate two commands written
on a single line.
The for loop begins with the formula
for <variable> in <group to iterate over>
. In
this case, the word filename
is designated as the variable
to be used over each iteration. In our case SRR097977.fastq
and SRR098026.fastq
will be substituted for
filename
because they fit the pattern of ending with .fastq
in the directory we’ve specified. The next line of the for loop is
do
. The next line is the code that we want to execute. We
are telling the loop to print the first two lines of each variable we
iterate over. Finally, the word done
ends the loop.
After executing the loop, you should see the first two lines of both fastq files printed to the terminal. Let’s create a loop that will save this information to a file.
When writing a loop, you will not be able to return to previous lines once you have pressed Enter. Remember that we can cancel the current command using
- Ctrl+C
If you notice a mistake that is going to prevent your loop for executing correctly.
Note that we are using >>
to append the text to
our seq_info.txt
file. If we used >
, the
seq_info.txt
file would be rewritten every time the loop
iterates, so it would only have text from the last variable used.
Instead, >>
adds to the end of the file.
Using Basename in for loops
Basename is a function in UNIX that is helpful for removing a uniform
part of a name from a list of files. In this case, we will use basename
to remove the .fastq
extension from the files that we’ve
been working with.
We see that this returns just the SRR accession, and no longer has the .fastq file extension on it.
OUTPUT
SRR097977
If we try the same thing but use .fasta
as the file
extension instead, nothing happens. This is because basename only works
when it exactly matches a string in the file.
OUTPUT
SRR097977.fastq
Basename is really powerful when used in a for loop. It allows to access just the file prefix, which you can use to name things. Let’s try this.
Inside our for loop, we create a new name variable. We call the
basename function inside the parenthesis, then give our variable name
from the for loop, in this case ${filename}
, and finally
state that .fastq
should be removed from the file name.
It’s important to note that we’re not changing the actual files, we’re
creating a new variable called name. The line > echo $name will print
to the terminal the variable name each time the for loop runs. Because
we are iterating over two files, we expect to see two lines of
output.
Exercise
Print the file prefix of all of the .txt
files in our
current directory.
One way this is really useful is to move files. Let’s rename all of
our .txt files using mv
so that they have the years on
them, which will document when we created them.
BASH
$ for filename in *.txt
> do
> name=$(basename ${filename} .txt)
> mv ${filename} ${name}_2019.txt
> done
Exercise
Remove _2019
from all of the .txt
files.
Key Points
-
grep
is a powerful search tool with many options for customization. -
>
,>>
, and|
are different ways of redirecting output. -
command > file
redirects a command’s output to a file. -
command >> file
redirects a command’s output to a file without overwriting the existing contents of the file. -
command_1 | command_2
redirects the output of the first command as input to the second command. -
for
loops are used for iteration. -
basename
gets rid of repetitive parts of names.