You can use simple unix functions such as grep ...
or use jMHC http://code.google.com/p/jmhc/
or

FlexBar http://seqanswers.com/wiki/Flexbar

Software list: http://seqanswers.com/wiki/

Thank you very much. Just a few "dummy" questions..
The file that we get from Miseq after decoding of the illumima index is in the format of a fastaQ file. As a clinician who is at complete loss when it comes to bioinformatics and running scripts, the programme that I am looking for is something into which we can input the fastQ files and then input the nt sequence of the codes, preferably on a webinterface and which would give the decoded format in preferably a fasta file. jMHC seems to fit the criteria a lot however, their input requirement is a fasta file. Has anyone tried jMHC for data other than MHC related and using fastQ to fasta converted files? Thank you..

convert using Galaxy web portal https://main.g2.bx.psu.edu

However..... If you are to embark on next generation sequencing data analysis there really is no way around knowing the basics of Unix/Linux and command line programs.
These are much more powerful that GUIs and can make your life MUCH MUCH easier.
A good place to start :http://korflab.ucdavis.edu/Unix_and_Perl/index.html

For example: jMHC ~ around 10 times faster on a Mac than PC...I have no idea why. But when I open jMHC on my Mac I do so from the terminal. This is so I can allocate more memory to Java (which jMHC runs in) so it can process my large data sets.
I do this by typing :

$ cd Desktop/jMHC
$ java -Xmx4g -jar jMHC.jar

This opens jMHC using 4gb RAM. If I do not do this jMHC will either freeze or crash on large data sets ~1M reads

It does not matter what amplicon you want to de-multiplex. jMHC was named so just because the group work on MHC.