This greatly depends on the assembler, and the specific depth and error rate, and what you are assembling (single-cell, metagenome, isolate, transcriptome, etc), repeat content, and more.

Metagenomes, transcriptomes, single-cells, and highly-repetitive isolates tend to be the most difficult (possibly in that order). The more highly variable your coverage is - whether due to community composition, amplification, gene expression, or repeats - the harder it is to tell the difference between low-coverage genomic sequence and error kmers. Some assemblers are better at this than others.

Informatically, the signal-to-noise ratio is more important than raw coverage. However, coverage is discrete so if you have 2X coverage with some errors, you will probably get a better assembly than with 1X coverage and no errors, since that has no overlaps and cannot possibly assemble, even though it has a better SNR.

In other words, there are no strict rules about whether it is good to increase coverage at the expense of accepting reads with higher error rates; you can find scenarios with directly contradictory best practices. Only once you decide on a specific sequencing platform, experiment type, organism, assembler, and sequencing volume, is it possible to objectively answer the question.