How can I make sure that the lane index is included in the STARsolo count matrix barcodes list?

If I run CellRanger and STARsolo on the same set of FASTQs I get full barcodes in CellRanger output:

(base) [mkarikom@gl1515 mkarikom]$ zcat 2024-05-14_rxn1_S1_Cellranger/outs/raw_feature_bc_matrix/barcodes.tsv.gz|head
AAACCAAAGAAACCAA-1
AAACCAAAGAAACCCC-1
AAACCAAAGAAACGGT-1
AAACCAAAGAAAGGTC-1
AAACCAAAGAAAGTCA-1
AAACCAAAGAAATCAG-1
AAACCAAAGAAATGGC-1
AAACCAAAGAAATTGG-1
AAACCAAAGAACAGAC-1
AAACCAAAGAACAGGT-1

But STARsolo is only reporting the nucleotide sequence without the lane index:

(base) [mkarikom@gl1515 mkarikom]$ head 2024-05-14_rxn1_S1_Solo.out/Gene/raw/barcodes.tsv
AAACCAAAGAGTACGG
AAACCAAAGATTCAGT
AAACCAGCAAGCTGGG
AAACCAGCACCGTTAG
AAACCATTCAATGCGC
AAACCCATCAATATTG
AAACCCATCCACTACT
AAACCCATCCCTGATT
AAACCCATCCGACTAA
AAACCCATCGGCTCTC

Where are you getting the info that the -1 corresponds to the lane? Because it doesn't.

From the 10X site:

The cell barcode CB tag includes a suffix with a dash separator followed by a number: AAACCCAAGGAGAGTA-1 This number denotes the GEM well, and is used to virtualize barcodes in order to achieve a higher effective barcode diversity when combining samples generated from separate GEM well channel runs. Normally, this number will be "1" across all barcodes when analyzing a sample generated from a single GEM well channel. It can either be left in place and treated as part of a unique barcode identifier, or explicitly parsed out to leave only the barcode sequence itself.

So more than likely, that suffix (or lack thereof) isn't providing you any additional info.

If you combine two samples together, the -1 and -2 at the end of cell barcodes will matter, so you know what cells came from what samples, especially because there is a non-zero chance that two different samples will have a few cells that happen to share the same cell barcode.